Post on 05-Mar-2020
1
ENHANCMENT OF LIPASE CATALYZED ISOAMYL ACETATE SYNTHESIS BY HIGH HYDROSTATIC PRESSURE AND USE OF ALTERNATIVE SOLVENTS
By
MICHAEL JOSEPH EISENMENGER
A DISSERTATION PRESENTED TO THE GRADUATE SCHOOL OF THE UNIVERSITY OF FLORIDA IN PARTIAL FULFILLMENT
OF THE REQUIREMENTS FOR THE DEGREE OF DOCTOR OF PHILOSOPHY
UNIVERSITY OF FLORIDA
2009
2
© 2009 Michael Joseph Eisenmenger
3
To my lovely wife, mother, father, and all my family and friends who helped,
encouraged, and guided me through my pursuit of a higher education. Without whom I could not have achieved my goals.
4
ACKNOWLEDGMENTS
I thank all those who helped me throughout my academic career, including: my
family Tom and Kerry, Pat and Lindsay, David and Rachel, Karen and Greg, and Leslie
and Rusty; my wife Caitlin; my academic advisor Dr Reyes; and my graduate committee
members Dr Preston, Dr Rouseff, Dr Marshall, and Dr Goodrich. Also special thanks to
my lab group Juan, Narsi, Rosy, and Shelley for all your help. Lastly, I acknowledge all
the assistance provided to me from the University of Florida, the Institute of Food and
Agricultural Sciences, the department of Food Science and Human Nutrition, and the
Citrus Research and Education Center who without any of this could not have been
possible.
5
TABLE OF CONTENTS
Page
ACKNOWLEDGMENTS .................................................................................................. 4
LIST OF TABLES ............................................................................................................ 8
LIST OF FIGURES .......................................................................................................... 9
LIST OF ABBREVIATIONS ........................................................................................... 11
ABSTRACT ................................................................................................................... 13
CHAPTER
1 INTRODUCTION .................................................................................................... 17
History ..................................................................................................................... 17
Overview of Current Enhancement Techniques/Technologies ............................... 19 Mechanisms of Pressure-Induced Stabilization ...................................................... 20 Mechanisms of Pressure Induced Activation .......................................................... 23
Enzymes Enhanced by High Pressure.................................................................... 28 Oxioreductases (EC. 1) .................................................................................... 29
Transferases (EC 2) ......................................................................................... 33 Hydrolases (EC 3) ............................................................................................ 34 Lyases (EC 4) ................................................................................................... 53
Remaining Challenges ............................................................................................ 53 Specific Objectives ................................................................................................. 54
2 HIGH HYDROSTATIC PRESSURE INCREASED STABILITY AND ACTIVITY OF IMMOBIILZED LIPASE IN HEXANE ................................................................. 57
Introduction ............................................................................................................. 57 Materials and Methods............................................................................................ 59
Materials ........................................................................................................... 59
Methods............................................................................................................ 60 Results and Discussion........................................................................................... 65
Effect of HHP on Lipase Stability ...................................................................... 65 Comparison of Pressurization and Heating Methods on Activation Energy ...... 68
Activation Volume Determination ..................................................................... 70 Electron Microscope Examination of Immobilization Beads ............................. 74
Conclusions ............................................................................................................ 76 Acknowledgments ................................................................................................... 77
3 ACTIVATION VOLUME AND APPARENT MICHAELIS MENTEN PARAMETERS OF LIPASE AT HIGH HYDROSTATIC PRESSURE IN HEXANE WITH EXCESS ALCOHOL ..................................................................... 82
6
Introduction ............................................................................................................. 82
Materials and Methods............................................................................................ 82 Materials ........................................................................................................... 82
Methods............................................................................................................ 84 Results and Discussion........................................................................................... 85
Activation Volume ............................................................................................. 85 Michaelis-Menten Parameters .......................................................................... 87
Conclusions ............................................................................................................ 90
Acknowledgments ................................................................................................... 91
4 ENHANCMENT OF NATURAL FLAVOR SYNTHESIS USING HIGH PRESSURE AND AN IONIC LIQUID-ALCHOL BIPHASIC MEDIA ........................ 94
Introduction ............................................................................................................. 94
Materials and Methods............................................................................................ 96 Materials ........................................................................................................... 96
Methods............................................................................................................ 97 Results and Discussion......................................................................................... 100
Qualitative Observations ................................................................................ 100 Conversion with Free and Immobilized Lipase ............................................... 100 Determination of Activation Energy ................................................................ 101
Determination of Activation Volume ............................................................... 103 Conclusions .......................................................................................................... 106
Acknowledgements ............................................................................................... 106
5 IN-SITU ANALYSIS OF LIPASE STRUCTURAL CHANGES INDUCED BY HIGH PRESSURE AND THERMAL TREATMENT ............................................... 112
Introduction ........................................................................................................... 112 Materials and Methods.......................................................................................... 113
Materials ......................................................................................................... 113 Results and Discussion......................................................................................... 115
Conclusions .......................................................................................................... 116 Acknowledgements ............................................................................................... 116
6 COMPREHENSIVE RESULTS, DISCUSSION, AND FUTURE STUDIES ........... 119
APPENDIX
A PICTURE OF HIGH HYDROSTATIC PRESSURE SYSTEM ............................... 123
B PICTURE OF HIGH HYDROSTATIC PRESSURE IONIC LIQUID REACTION VIAL ...................................................................................................................... 124
C PICTURE OF HIGH HYDROSTATIC PRESSURE OPTICAL CELL ..................... 125
LIST OF REFERENCES ............................................................................................. 126
7
BIOGRAPHICAL SKETCH .......................................................................................... 147
8
LIST OF TABLES
Table page 2-1 Initial rate and percent change using various “pressure first”, “heat first”, and
“simultaneous” methods of applying heat and pressure as compared to assays at low pressure. ...................................................................................................... 81
3-1 Activation volume using the Eyring equation at 40 and 80 °C for lipase catalyzed production of isoamyl acetate. ± Values represent the standard error of the linear regression used in determination of activation volume. ................................. 93
3-2 Michaelis-Menten kinetic parameters KM (mmol L-1) and Vmax (mmol L-1 s-1) of lipase catalyzed isoamyl acetate formation in hexane at 40 or 80 ˚C and 0.1 or 200 MPa. The ± values represent standard error from linear regression. ............... 93
4-1 Activation energy (Ea) of free and immobilized lipase at 0.1 or 300 MPa .............. 111
9
LIST OF FIGURES
Figure page 1-1 Theoretical generic elliptical pressure versus temperature diagram with native
and denatured protein regions inside and outside of the ellipse respectively, separated by a zone of reversible denaturation. ..................................................... 56
2-2 Temperature (circle) and pressure (triangle) profiles for (A) “Pressure-First”, (B) “Simultaneous”, and (C) “Heat-First” method for a 10 minute incubation at 80 °C and 400 MPa. ......................................................................................................... 77
2-3 Effect of high pressure on enzyme stability after incubation for 4 h at 80 °C. Assayed with 10 ± 0.5 mg lipase, 0.06 M substrate. Error bars represent a 95% confidence interval using analysis of variance. ....................................................... 78
2-4 Effect of pressure on Vmax at (●) 40 °C and (■) 80 °C for lipase-catalyzed production of isoamyl acetate (Novozyme 435 in n-hexane ) using the “pressure-first method”. Error bars represent standard error of the slope of apparent the initial rate calculated from linear regression using a 95% confidence intervals. ............................................................................................... 79
2-5 Determination of activation volume using the Eyring equation at (●) 40 and (■) 80 °C for lipase catalyzed production of isoamyl acetate using the “pressure-first method”. ........................................................................................................... 79
2-6 Scanning electron micrographs of the surface of Lipozyme® (Novozyme L4777) immobilized on acrylic resin (A) before and (B) after exposure to hexane solvent at 80 °C and 700 MPa for 4 h and after assay (C) without incubation and (D) with incubation at 80 °C and 700 MPa for 4 h treatment. Inserts illustrate the retention of bead integrity after different treatments. .............................................. 80
3-1 Temperature (○) and pressure (▲) profiles using the “pressure-first” method at 80 ˚C and 400 MPa. ................................................................................................ 91
3-2 Kinetic mechanism (Ping Pong Bi Bi) of lipase-catalyzed synthesis of isoamyl acetate from acetic acid and isoamyl alcohol using Cleland’s notation where E represents free enzyme and E* is the activated enzyme state. .............................. 91
3-3 Effect of pressure on Vmax at (●) 40 °C and (■) 80 °C for lipase-catalyzed production of isoamyl acetate (Novozyme 435 in n-hexane). Error bars represent standard error of the slope of apparent initial rate calculated from linear regression using a 95% confidence interval. ................................................. 92
3-4 Linearized effect of pressure on V0 according to Eyring equation at (●) 40 and (■) 80 °C for lipase catalyzed production of isoamyl acetate. ................................. 92
10
3-5 Lineweaver-Burk plot of isoamyl acetate production at (♦) 0.1 MPa and 40 ˚C, (■) 200 MPa and 40 ˚C, (▲) 0.1 and 80 ˚C, and at (●) 200 MPa and 80 ˚C. Rate is expressed as mmol isoamyl acetate L-1 s-1 while substrate concentration is expressed as mmol L-1 acetic acid. ......................................................................... 93
4-1 Depiction of the custom made IL-HHP reaction vial. ............................................. 107
4-2 Reaction vessels with ionic liquid biphasic mixture and free lipase. ...................... 107
4-3 Concentration (mM) of isoamyl acetate produced by CALB (7.5 U/ml) in an IL-alcohlic biphasic system at 40 ˚C. Error bars represent standard deviation of three replicates. .................................................................................................... 108
4-4 Concentration (mM) of isoamyl acetate produced after 3 h incubation per unit enzyme of free CALB at (grey) 0.1 or (black) 300 MPa. Error bars represent standard deviation of three replicates. .................................................................. 108
4-5 Concentration (mM) of isoamyl acetate produced after 3 h incubation per unit enzyme of immobilized CALB at (grey) 0.1 or (black) 300 MPa. Error bars represent standard deviation of three replicates. .................................................. 109
4-6 Apparent initial rate per unit enzyme of free CALB at (○) 0.1 or (□) 300 MPa. Error bars represent standard error of linear regression. ...................................... 109
4-7 Determination of activation energy using the Arrhenius equation at (◊) 0.1 and (□) 300 MPa. ......................................................................................................... 110
4-8 Apparent initial rate per unit enzyme of free CALB at (○) 40 or (□) 80 ˚C. Error bars represent standard error of linear regression of five data points. .................. 110
4-9 Determination of activation volume using the Eyring equation at (◊) 40 and (□) 80 °C. .................................................................................................................... 111
5-1 Schematic representation of the high pressure optical cell with sapphire windows and fiber optic ports for continuous optical measurements in situ. ......... 117
5-2 Intensity expressed in counts of fluorescence at 350 nm emitted from lipase during 3 cycles of pressurization (0.1 to 500 MPa), heating (10 ˚C to 80 ˚C), and 2 minute incubations followed by cooling and depressurization. ........................... 118
11
LIST OF ABBREVIATIONS
HP High pressure
HHP High hydrostatic pressure
HPT High pressure treatment
SC-CO2 Supercritical carbon dioxide
BPTI Bovine pancreatic trypsin inhibitor
NMR Nuclear magnetic resonance
GAPDHs Glyceraldehyde-3-phosphate dehydrogenase
GDH Glutamate dehydrogenase
YADH Yeast alcohol dehydrogenase
TBADH Thermoanaerobium brockii alcohol dehydrogenase
POD Peroxidase
LOX Lipoxygenase
PPO Polyphenoloxidase
PCR Polymerase chain reaction
PME Pectin methylesterase
SCSF5 Sulfur hexafluoride
CALB Candida antarctica lipase B
CALA Candida antarctica lipase A
Ea Activation Energy
SEM Scanning electron microscope
PG Polygalacturaonase
GRAS Generally recognized as safe
CT Alpha-chymotrypsin
12
BLG Beta-lactoglobulin
13
Abstract of the Dissertation Presented to the Graduate School of the University of Florida in Partial Fulfillment of the Requirements for the Degree of Doctor of Philosophy
ENHANCMENT OF LIPASE CATALYZED ISOAMYL ACETATE SYNTHESIS BY HIGH
HYDROSTATIC PRESSURE AND USE OF ALTERNATIVE SOLVENTS
By
Michael Joseph Eisenmenger
December 2009
Chair: José I. Reyes-De-Corcuera Major: Food Science and Human Nutrition
While most current applications of high pressure (HP) are for inactivating
deleterious enzymes, there is evidence that high pressure can induce stabilization and
activation of some enzymes. Various other strategies have been employed to enhance
enzyme stability, including; genetic engineering, immobilization, and operating in non-
aqueous media. While each of these strategies has provided varying degrees of stability
or activity enhancement, the application of high pressure may be a complementary,
synergistic, or an additive enzyme enhancement technique. Over 25 enzymes that have
exhibited high pressure stabilization and/or activation were compiled. Each enzyme
discussed responds differently to high pressure depending on the pressure range,
temperature, source, solvent or media, and substrate. Possible mechanisms for
pressure-induced stabilization and activation are discussed and compared with current
enzyme enhancement techniques.
Lipases are the most widely used enzyme in high value product synthesis,
modification, and enhancement. However, they are often unstable above 40 °C. Isoamyl
acetate has a banana flavor and is widely used. When synthesized from a lipase-
14
catalyzed reaction it can be considered a “natural” flavor ingredient. This study
examines the apparent kinetics of immobilized lipase-catalyzed synthesis of isoamyl
acetate at HHP in hexane. HHP reduced thermal inactivation of lipase by up to 152%
after 4 h at 80 °C and 400 MPa when compared to incubations at low pressure. No
significant differences were found in activation energy (Ea) at different pressures,
regardless of the pressurization and heating sequence, and were between 35.7 ± 3.5
and 47.8 ± 8.2 kJ mol-1, depending on the method. In all methods utilized, activity at
63.5 and 80 °C at 400 MPa was greater (from about 20 to 96% increase) than at low
pressure. Activity increased by 110% at low pressure versus a 239% increase at 350
MPa when the temperature was increased from 40 to 80 °C. Increasing pressure up to
350 MPa increased lipase activity while pressures greater than 350 MPa maintained or
decreased lipase activity. Activation volume (ΔV≠) appeared negative between ambient
pressure and 200 MPa in contrast to a positive ΔV≠ between 300 and 600 MPa.
Apparent ΔV≠ was 14.3 or 15.2 ± 2.2 cm3 mol-1 at 40 or 80 °C, respectively, between
300 and 500 MPa.
This study also examines further the negative and positive activation volumes
(ΔV‡) and Michaelis-Menten parameters (KM and Vmax) of immobilized lipase-catalyzed
synthesis of isoamyl acetate at HHP in hexane. At 80 ºC Vmax increased (negative ΔV‡)
from 10 to 250 MPa, remained relatively constant between 250 and 350 MPa, then
decreased (positive ΔV‡) from 350 to 600 MPa. At 40 ºC Vmax increased (negative ΔV‡)
from 1 to 100 MPa, remained relatively constant between 100 to 200 MPa, and then
decreased (positive ΔV‡) from 200 to 600 MPa. Temperature affected ΔV‡ at low
pressure but did not at high pressure; indicating that pressure induced activation is
15
affected by temperature while inactivation is not. Pressure significantly increased Vmax
at both temperatures by approximately 1-log, however pressure only affected KM at 40
˚C but not at 80 ˚C. Increased KM indicates that the enzyme substrate complex
formation is being hindered at 40 ˚C but not at 80 ˚C. The Vmax was lower at 80 ˚C and
low pressure than at 40 ˚C and 200 MPa which may be attributed to lipase inactivation
at high temperatures and low pressures.
The application of high hydrostatic pressure (HHP) on the apparent kinetics of
immobilized and free lipase (Candida antarctica lipase B) in a biphasic ionic liquid (IL)-
alcohol system was investigated. ILs have become an attractive alternative media
because they can enhance stability, enantioselectivity, product yield, and reaction rate
of enzyme reactions. Although the application of IL and HHP to enzyme catalysis has
been previously explored separately, this study is the first to explore the combination of
these technologies. Production of isoamyl acetate was up to 10-fold higher with free
lipase versus immobilized lipase after 3 h at 300 MPa and 80 ˚C. Rate of catalysis by
free lipase also increased up to 15 and 25-fold at 500 MPa versus at 0.1 MPa at 40 or
80 ˚C, respectively. Pressure affected the activation energy (Ea) of immobilized lipase
but not free lipase (43.4 ± 3.1 and 55.4 ± 0.1 kJ mol-1 at 0.1 and 300 MPa respectively).
Temperature had no effect on activation volume (ΔV‡) which was -16.1 ± 1.5 and -16.7
± 1.4 cm3 mol-1 at 40 and 80 ˚C respectively. It was also observed that after treatment at
high pressure, the free lipase is temporarily suspended in a semi-solid IL phase. This
“temporary immobilization” has not been previously described, and may be useful in
aiding the separation of phases between reaction cycles.
16
This study has demonstrated how high pressure can induce activation and
stabilization of lipase in a variety of solvents. However, there is a significant lack of data
describing the continuous in situ conformational changes induced by combinations of
temperature and pressure that may be causing activation and/or stabilization.
Fluorescence spectroscopy has been conducted in situ at pressures up to 500 MPa and
up to 80 ˚C. Results indicate immediate and profound changes in tryptophan
fluorescence as indicated by changes in the intensity at 350 nm. Although these results
are qualitative, they do provide a valuable insight into the conditions which trigger
conformational changes.
17
CHAPTER 1 INTRODUCTION
History
In June of 2007, the scientific community celebrated the 30th anniversary of the
discovery of volcanic hot vents at the Galapagos Rift at the bottom of the Pacific Ocean.
The most notable finding was not the vent itself, but the abundance of entire
ecosystems at these extreme conditions (up to 120 MPa, 2–100 ˚C, absence of
sunlight, and scarce supply of organic nutrients) which led to a fundamental change in
our understanding of life on Earth. While the presence of barophilic (also termed
piezophilic) bacteria was first hypothesized in 1949 [1] and later discovered in various
trenches during the Galathea Deep-Sea Expedition of 1950-1952 [2] , this was the first
discovery of multi-cellular life in the deep sea. These discoveries spawned a global
quest for life from extreme conditions. This search has resulted in the discovery of over
550 species thriving at various extreme pressures and temperatures and new species
continue to be discovered at a rate of about two per month in environments as extreme
as 470 ˚C [3]. Discoveries of both thermostable and piezostable microorganisms and
their enzymes have enabled the field of high pressure enzyme modification to progress
dramatically by uncovering several high pressure-induced enzyme applications [4] and
modifications.
Since the discovery of microorganisms in deep-sea sediments [5, 6] in the 1880’s,
high pressure (HP) and its application to bioscience was only briefly demonstrated in
the early 1900’s [7]. While HP was effective at inactivating various deleterious enzymes
[8-14], its effect on enzyme stabilization and activation was explored less extensively [4,
15-19]. Enzymes from mesophilic and extremeophilic microorganisms were stabilized
18
by HP [20, 21]. Extremophiles are defined as organisms that have evolved to exist in
extreme environments and fall into at least 15 classes of which the most common are
thermophiles, acidophiles, alkalophiles, psychrophiles, and barophiles, among others
[22]. Within the context of this review, thermophilic organisms will be sub-categorized
into moderate thermophiles (45-65 ˚C), thermophiles (65-85 ˚C), hyperthermophiles (85-
100 ˚C), and extreme thermophiles (>100 ˚C).
Extremely heat-tolerant (stable up to 150 ˚C) enzymes have potential application
in organic media [22-24]. However, the boiling point of most organic solvents is well
below 100 ˚C. As pressure is raised, the boiling point of organic solvents increases
allowing studies above conventional temperatures at 0.1 MPa [25]. The ability to
operate with organic or volatile solvents at temperatures above their conventional
boiling point is an important yet often overlooked advantage of HP.
The cost of high pressure processing (HPP) decreased over the last decade and
become more widely implemented particularly in the food industry. In 2007 there were
about 120 HPP industrial installations operating worldwide [26] with 80% of their
equipment installed since 2000. HPP food became a two billion dollar global market and
is expected to comprise 450 million pounds/year in 2008 [27]. As demand for HPP
equipment grows, innovation is expected to continue to reduce capital and operating
costs [26]. Although HPP of bulk foods is currently more widespread, the much higher
profit-margin sector of enzyme catalyzed synthesis of high added-value products such
as pharmacological peptides, antibiotics, carbohydrates, and food flavors has greater
potential for adopting HPP.
19
The effects of HP on proteins and enzyme inactivation was discussed and
reviewed over the past 20 years [16, 18, 19, 28-31]. Theories of pressure effects on
enzymes and the activation volumes of several enzymes were compiled in the early
1980’s [32]. However, the application of HP to enhance enzyme catalysis has not been
extensively explored or comprehensively reviewed.
Overview of Current Enhancement Techniques/Technologies
The major drawback to the extensive use of many enzymes compared to chemical
catalysts is their relatively low stability in their native state and their often prohibitive
cost [33]. There is a great interest in developing competitive biocatalysts for industrial
applications by improvement of their activity, stability, and re-usage capacity. Such
improvements have been approached by chemical, physical, or genetic modification of
the native enzyme. The effects of immobilization on activity, stability, and even
selectivity of some enzymes have been well documented [34-36]. For example,
immobilization of lipase can improve activity by shifting the equilibrium between open
and closed form towards the open, more active form [35]. Also, chymotrypsin can be
stabilized by a factor of 60,000 by immobilization [37]. Furthermore, the enantiomeric
ratio of lipase products may be changed from 1 to almost 100 by using different
immobilization preparations [35]. Furthermore, modification of the reaction environment
was explored using alternative solvents including organic solvents such as hexane [38-
41], solvent-free systems [42-48], dense or supercritical gases such as supercritical
carbon dioxide (SC-CO2) [49-51], and more recently ionic liquids [52-54]. For example,
stability and selectivity of lipase in ionic liquid increased 2.7-fold and by 2%,
respectively, when compared to in hexane [54]. Likewise, lipase activity dramatically
increased in SC-CO2 with a negative activation volume of 1340 cm3 mol-1 [55].
20
Enzymes suitable for use in industrial biocatalysis may require application of a
combination of these improvement methods.
Mechanisms of Pressure-Induced Stabilization
Although the mechanisms of HP-induced stabilization has yet to be fully
elucidated, it appears that intramolecular interactions, hydration of charged groups,
disruption of bound water, and stabilization of hydrogen bonds may all play a role. The
pressure effects on intra- and intermolecular interactions within proteins were reviewed
in depth [56].
According to Mozhaev et al. [57], a possible explanation of pressure-induced
stabilization of enzymes against thermal inactivation rests in opposing effects of
pressure and temperature on the ability of protein functional groups to interact with
water. The promotion of charged species in aqueous medium is favored by a high-
pressure environment, because the electrostriction of water around the charges
decreases the molar volume of water [58]. This means that an increase in pressure will
weaken the electrostatic or coulombic interactions. Hydration of charged groups by
water molecules is strengthened by pressure and weakened at high temperature [18,
28]. Evidence of this phenomenon was presented by Kitchen et al. [59] who completed
a molecular dynamics simulation of bovine pancreatic trypsin inhibitor (BPTI) in solution
at HP and found large pressure-induced changes in the structure of the hydration shell,
the shell appeared more ordered at HP, and that HP-induced greatest ordering for
nonpolar surface groups. Enzymatic catalysis in organic media also depends on
enzyme hydration state which is greatly influenced by pressure [60]. Mozhaev et al. [57]
hypothesized that, at an initial step of thermal inactivation, a protein loses a number of
essential water molecules, and this loss may give rise to structural rearrangements in a
21
protein. HP may hamper this process by favoring hydration of both charged and
nonpolar groups. In other words, application of high hydrostatic pressure fortifies the
protein hydration shell thus preventing thermal inactivation.
Hydrogen bonding may also be slightly strengthened by an increase in pressure,
because of, according to Kunugi [58], the decrease in the inter-atomic distance leading
to a smaller molecular size. This phenomenon was initially based on the negative
activation volumes associated with hydrogen bond formation in organic compounds
such as formic acid, ε-caprolactam, phenol, and poly-L-lysine [61]. Later, the lengths of
existing hydrogen bonds within proteins have been observed to be shorter under HP as
first detected by nuclear magnetic resonance (NMR) [62, 63] and then by low-frequency
Raman spectroscopy [64].
Hydrophobic interactions also greatly affect enzymatic conformation. The
relationship between HP and temperature effects on hydrophobic interactions has yet to
be fully understood [56]. It was suggested that hydrophobic interactions are
strengthened by HP because the hydration of non-polar surface molecules is not
favored due to the corresponding volume increases [30, 65]. Evidence supporting this
hypothesis was provided by Hei and Clark [66] by demonstrating how the stability of
several glyceraldehydes-3-phosphate dehydrogenases (GAPDHs) with varying
hydrophobicity of their “s-loops” (structural motifs consisting of residues 178 to 201
which are an important determinant of GAPDH thermal stability) is correlated to
pressure-induced stabilization. Further evidence was provided by Mei et al. [67] who
studied the role of hydrophobic residues on pressure-induced stabilization. Through
site-directed mutagenesis, Mei et al. [67] modified the hydrophobicity of azurin and
22
pressure-induced stabilization increased with increasing hydrophobicity. However, this
was in disagreement with Mozhaev et al. [18] who said “it is generally accepted that
formation of hydrophobic contacts proceeds with positive ΔV≠ and is therefore
disfavored by pressure” and cited the formation of hydrophobic interactions when
transferring methane from a non-polar solvent to water, the micelle formation by
surfactants, and a dimerization of carboxylic acid [68, 69] which all resulted in a positive
ΔV≠. However the dimerization of formic, acetic, propionic, and n-butyric acid all had
negative ΔV≠ [69].
Pressure and heat are generally thought to be antagonistic factors in molecular
terms (from the principle of microscopic ordering, an increase in pressure at constant
temperature leads to an ordering of molecules or a decrease in the entropy of the
system) and more recently with regards to enzyme conformation within defined
pressure and temperature regions [17-19, 28]. This defined region must be determined
experimentally as the complexity of using an enzyme catalyst prevents accurate
modeling without pre-determination of enzyme stability and activity at various pressure-
temperature combinations. The relationship between pressure and temperature effects
on enzyme conformation often results in an elliptical pressure versus temperature
diagram as shown in Fig. 1 with native and denatured protein regions inside and outside
of the ellipse, respectively, separated by a zone of reversible denaturation with the
contour line representing where the equilibrium concentrations of native and denatured
forms of the enzyme are equal.
A comprehensive review of pressure-temperature phase diagrams of protein
unfolding was compiled by Smeller [70]. Increases in temperature and pressure can
23
have both, stabilizing or denaturing effects on enzymes depending on the initial
conditions, as represented by points A, B, C, and D in the elliptical diagram and the
magnitude of the increase. For example, moderately increasing temperature and
pressure from point A stabilizes the enzyme. However, in point D, increases in both,
temperature or pressure destabilizes the enzyme. In the case of point B an increase in
pressure denatures the enzyme but an increase in temperature stabilizes it and vice-
versa for point C. Such diagrams were first shown by Hawley [71] and later reviewed
and discussed by several others [16, 17, 70, 72]. However, they are typically
representations of the rate of denaturation which doesn’t always directly correlate to
inactivation. These diagrams have been used to describe pressure stability of
chymotrypsin [71], polyphenoloxidase [73, 74], pectin methylesterase [75-77],
myrosinase [78], naringinase [79], β-glucanase [80], α and β-amylase [81, 82], and
glucoamylase [83].
Mechanisms of Pressure Induced Activation
Explanations for pressure-induced changes in the rate of enzyme-catalyzed
reactions can be classified into: (1) direct changes in the structure of an enzyme, (2)
changes in the reaction mechanisms; for example, a change in the rate-limiting step,
and (3) changes in the substrate or solvent physical properties (e.g. pH, density,
viscosity, phase) that affect enzyme structure or the rate-limiting step.
Early studies suggested that the activities of monomeric enzymes activity was
stimulated, while the activities of multimeric enzymes were inhibited by application of
high hydrostatic pressure [56]. However, at least 15 dimeric and tetrameric enzymes
have been reported to be activated by pressure [32].
24
It is understood that pressure effects on reaction rates adhere in most cases to Le
Châtelier’s principle: that elevated pressures favor changes that reduce a systems’
overall volume. Thus, by comparing the total volumes of the reactants versus products,
of the ground state versus activated state, or of the dissociated versus bound complex,
the effect of pressure on reaction rate and equilibrium can be estimated [28] using the
Eyring equation (Eq. 1-1) [57],
(1-1)
where p is the pressure, T is the absolute temperature, R is the ideal gas constant, ΔV≠
is the activation volume that represents the dependence of the reaction rate with
pressure, and k is the rate constant. After integration and rearrangement, Eq. (1) can be
rewritten as Eq. (1-2).
(1-2)
where k0 is the rate constant at a reference pressure P0. Thus, any rate with a negative
volume change will be shifted toward the more compact state by increasing pressure
and any reaction with a positive activation volume will be slowed.
Compared to chemical catalysis, it is more difficult to give a precise physical
meaning to ΔV≠ for enzyme reactions because pressure affects several factors
including: enzyme conformation, enzyme solvation (interaction with surrounding
medium, other proteins, water, ions, etc.), chemical equilibrium, and changes in
immobilization support or immobilization bonding. Depending on the reaction or
25
conformational changes of the enzyme (which are dependent on the temperature-
pressure range), activation volume can be positive, negative, or negligible. Typically
ΔV≠ ranges from -70 cm-3 mol-1 to + 60 cm-3 mol-1, with most having a magnitude of less
than 30 cm-3 mol-1 [28].
Separating the effects of HP on the rate constant from those on enzyme
conformation and thus on the availability of active enzyme at elevated pressures is
difficult because they both occur simultaneously affecting the rate of catalysis. The
simple one-substrate Michaelis-Menten mechanism and equation are shown in
equations 1-3 and 1-4.
PESESE
21
1
k
n
k
kn
(1-3)
(1-4)
where ET is the total enzyme concentration ([E]+[ES]), [S] is the substrate
concentration, v is the rate of reaction, and k1, k-1, and k2 represent rate constants and
KM is Michaelis-Menten constant. Large increases in pressure, temperature, or addition
of a denaturing agent causes the native enzyme (En) to first become reversibly (Er) and
then irreversibly (Ed) inactivated as described in Eq. (1-5). However, moderately
increasing pressure can produce a more active enzyme (Eact) as shown in Eq. (1-6)
which accounts for pressure induced activation.
(1-5)
26
(1-6)
The rate constant is also affected by temperature and generally expressed by the
Arrhenius equation (Eq. 1-7)
(1-7)
where Ea is the activation energy and kTo is the rate constant at a reference temperature
T0. Both temperature and pressure may be complementary to activation at a range of
temperatures and pressures; however, it can also hinder the reaction rate by
inactivating the enzyme. The combined effect of pressure and temperature is currently
impossible to predict without some preliminary data,
In the past 25 years, enzyme catalysis in organic media (mainly n-hexane) was the
focus of many studies and reviews [24, 39, 40, 58-65]. The pressure dependence of the
solubility parameter and molar volume of organic solvents was recently described at
pressures up to 300 MPa at 30 ˚C [66]. Pressure monotonically increased the solubility
parameter (~20%) and decreased the molar volume (16%) of many of the commonly
used organic solvents. Use of non-polar solvents results in better esterification (i.e.
higher conversion rates, increased stability, etc.) as they preserved the catalytic activity
without disturbing the aqueous mono-layer of the enzyme [67]. The pressure effect on
increasing polarity of organic (non-polar) solvents may hinder esterification as product
formation is favored in less polar solvents. However, the flexibility of some enzymes is
increased with increasing polarity of the organic solvent [68]. Therefore, pressure may
increase conformational flexibility, thus improving reaction rates as conformational
27
flexibility is required for activation of enzymes that show interfacial activation in the
presence of substrate.
Activity of lipase [41, 69], thermolysin [70], esterase (from Bacillus licheniformis)
[71], chymotrypsin [72, 73], xanthine oxidase [74, 75], horseradish peroxidase [76],
polyphenol oxidase [76], subtilisin [73], protease (from Bacillus subtilis) [73], and alcohol
dehydrogenase [77] are active in organic or non-aqueous media. Enzyme activity in
organic solvents can be correlated with the solvent polarity [40, 41, 78]. However it has
also been reported that activity might be affected by the solvent without correlation to
the polarity [79, 80]. It was suggested that enzymes that are active in organic solvents
retain their native structure upon transfer from water to organic solvents [73]. This is
evidenced by the phenomenon of pH memory discussed by Klibanov [76] which
suggests the presence of trapped active sites in organic solvents [64, 73] and the
observation that the addition of strong acids to lipase in hexane does not appreciably
inactivate the enzyme [81]. However, it is essential to have small amounts of water to
maintain stability and flexibility of lipases in organic solvent. Thus, enzyme-bound water
is essential for catalysis and serves as a “lubricant” for the enzyme [64, 73]. In contrast,
fully dry enzymes are inactive and enzymes in organic solvents with high amounts of
water show denaturation [64, 73]. Therefore, it is reasonable to hypothesize that
pressure-enhanced activity of enzymes in low or non-aqueous solvents may be partially
attributed to the pressure-induced hydration of charged groups.
Solvent compression at HP increases substrate molar concentration producing an
increase in reaction rate. Solvent compression also results in increased viscosity, which
in results in a decrease in reaction rate particularly in heterogeneous systems. Because
28
most enzymes utilized in organic media are immobilized (due to limited solubility),
viscosity effects may be significant unless adequate turbulence is provided.
The objective of this paper is to compile and critically present reports of HP
enzyme enhancement as an effective reaction parameter with potential for greater
utilization in enzyme catalysis.
Enzymes Enhanced by High Pressure
Discussion of the effects of pressure on enzyme stability and activity is organized
by enzyme commission (EC) number.
29
Oxioreductases (EC. 1)
Dehydrogenase (EC 1.1.1.1).
Dehydrogenases and hydrogenases are widely distributed in nature and have
been found in many microorganisms, plants, and animals and are the key enzyme
involved in the metabolism of H2. Studies in the 1960s with malic dehydrogenase from
Bacillus stearothermophilus had no activity at 101 ˚C from 0.1 to 70 MPa. However,
activity was induced above 70 MPa with optimal activity at 130 MPa at 101 ˚C [85]. This
relative activation was attributed to pressure counteracting the increased volume
associated with enzyme denaturation. HP effects on the oxidation of benzyl alcohol by
yeast alcohol dehydrogenase were measured by substrate capture. Moderate pressure
increased the rate of capture of benzyl alcohol 4-fold at 150 MPa and was attributed to
activating the hydride transfer step [84].
Pressures up to 75.9 MPa stabilized two glutamate dehydrogenases (GDH) from
the hypothermophile Pyrococcus furiosus and a recombinant GDH mutant [82]. The
stabilizing effects of pressure increased with temperature reaching 36-fold for
recombinant GDH at 105 ˚C and 75.9 MPa. Likewise, GDH from the liver of the
Antarctic fish Chaeonocephalus aceratus remained active up to 140 MPa and had
slightly increased activity from 2 to 100 MPa compared to 0.1 MPa, although reaction
rate decreased with pressure above 100 MPa [132]. Fish GDH was rapidly inactivated
above 200 MPa while bovine GDH was inactivated slowly in the range of 220-290 MPa
[132, 133].
Pressure inhibited the tetrameric mesophilic yeast alcohol dehydrogenase
(YADH), whereas the thermostable Thermoanaerobium brockii alcohol dehydrogenase
30
(TBADH) was activated by pressure up to 100 MPa [83]. These results supported the
hypothesis that HP can stabilize enzymes from thermophiles and that pressure
stabilization may be related to increased hydophobicity of surface groups typically
associated with thermophilic enzymes as discussed earlier in section 1.3. Furthermore,
differences in genetic sequences (Ala-180 and His-229) of dehydrogenases have been
discovered between two dehydrogenases from the same organism (Moritella sp. strain
2D2) found in vastly different pressure and temperature environments [134, 135] and
provided further evidence that pressure-induced stabilization or activation may be
related to a specific genetic sequence or set of sequences as discussed in section 1.3.
Hydrogenase (EC 1.1.1.2)
The relationship between thermophilicity and pressure stabilization was explored
using partially purified hydrogenases from a mesophile, Methanococcus maripaludis; a
moderate-thermophile, Methanococcus thermolithotrophicus; a hyper–thermophile,
Methanococcus igneus; and the extreme-thermophile deep-sea methanogen,
Methanococcus jannashii. HP from 1.0 to 50.7 MPa increased the half-life of the
hydrogenase from M. jannashii and M. ignius at 90 ˚C 4.8- and 4.5-fold, respectively,
while pressure decreased the half-life of M. thermolithotrophicus and M. maripaludis
[86]. Hydrogenase activity from M. jannashii more than tripled by an increase from 0.75
to 26 MPa at 86 ˚C with a corresponding ΔV≠ equal to -140 ± 32 cm3 mol-1 [87]. These
results further supported the hypothesis that barophilicity increases with thermophilicity.
Peroxidase (1.11.1.1-16)
Peroxidases (POD) constitute a group of thermostable heme proteins that oxidize
substrates (monophenols, diphenols, etc.) while utilizing H2O2 [136]. Although POD
often has a deleterious role in food quality, it can also be used as a catalyst in many
31
industrial applications, including; wastewater treatment, fine chemical biosynthesis, and
even paper pulp treatment [137]. While POD is widely used, its main limitations are
enzymatic stability and low production yield.
High pressure treatment (HPT) increased activity of strawberry POD by 13% and
1% at 400 MPa when applied for 5 and 10 min, respectively [88]. Similarly, crude extract
of mate tea leave POD increased activity 25% after exposure to compressed CO2 at 30
˚C and 7 MPa [136] and was attributed to the opposite effects of pressure and
temperature on the ability of the protein functional groups to interact with water. Carrot
and apple POD were also quite resistant to pressurization below 900 MPa for 1 min,
and activation was observed for treatments at 300-500 MPa [95].
Lipoxygenase (EC. 1.13.11.12)
Lipoxygenase (LOX) is a non-heme iron-containing dioxygenase that is found
throughout the plant kingdom, especially in legumes [89]. It causes chlorophyll
destruction and off-flavor development in frozen vegetables and is, therefore, a target
for inactivation. Green pea LOX demonstrated resistance to thermal inactivation above
60 ˚C under 200 MPa [89]. Likewise, LOX from soybean activity increased 120% after
treatment at 200 MPa and 55 ˚C for 15 min in 30% sucrose solution compared to
residual activity at 0.1 MPa [90]. Although LOX is generally considered a deleterious
enzyme in foods and a target for inactivation, pressure-induced stabilization or
activation provide further evidence toward the role of HP in enzyme enhancement.
Polyphenoloxidase (EC 1.14.18.1)
Polyphenoloxidases (PPO) are a group of copper proteins that catalyze the
oxidation of phenolics to quinones that produce brown pigments. They are widely
distributed in plants, animals, and microorganisms. The oxidation of phenolic substrates
32
by PPO is a major cause of browning in foods during ripening, handling, storage, and
processing. It is estimated that over 50% of losses in fruits occur as a result of browning
[138]. However, PPO is vital for the desirable color and flavor generation characteristic
of many plant based foods.
Mushroom PPO activity increased 140% after treatment at 400 MPa for 10 min
compared to untreated sample; and even after 10 min at 800 MPa about 60% residual
activity remained [93]. The enhancement in activity was hypothesized to be from
pressure-induced changes in the interactions with other constituents in the extract or
from the release of membrane-bound enzymes. Similarly, PPO from pears was
activated at 400 MPa with a maximum 5-fold increase activity at 600 MPa and 20 ˚C for
6 h [139]. Unlike the mushroom extract, PPO from pear showed pressure-induced
activation which could not be explained by interactions with other constituents as the
PPO was extracted and purified to homogeneity. It was suggested that such activation
is a result of a limited conformational change in the enzyme, release of the enzyme from
an enzyme-inhibitor complex, or activation via limited proteolysis such as zymogen
activation [140]. Asaka and others [140] concluded that PPO of La France pear fruit in
its latent form is activated by a limited conformation change; however, such a
mechanism is not known.
Victoria grape must PPO experienced a synergistic effect between pressure and
temperature for inactivation at 20 to 60 ˚C and 200 to 800 MPa and antagonistic effects
at above 60 ˚C and below 200 MPa [96]. Above 600 MPa, a temperature increase from
50 to 80 ˚C was needed to accelerate PPO inactivation by a factor of 10 [141]. Below
300 MPa, the inactivation rate constant decreased with increasing pressure which was
33
ascribed to the antagonistic effect of pressure and temperature [141]. A similar
antagonistic effect was observed for avocado PPO at high temperature (T ≥ 62.5 ˚C)
and low pressure (P ≤ 250 MPa) where a pressure increase caused a decrease in
inactivation rate [91]. It was also shown that avocado PPO exhibits HP stability (900
MPa for 270 min produced only 1 log-reduction of activity) at room temperature [91].
Red raspberry PPO was activated at 400 and 800 MPa by 15 and 8%, respectively [88].
Likewise, PPO cell-free extracts from carrots and apples showed a dramatic increase in
enzyme activity at pH 4.5 and 5.4 after pressurization at 100 to 300 MPa for 1 min [95].
The activation effects, observed for moderate pressure treatments was attributed to
reversible configuration and or conformation changes on enzyme and/or substrate
molecules [95].
Onion extract PPO activity increased up to 500 MPa with maximal activity of 142%
compared to untreated enzyme [92]. The mechanism of this pressure-induced
enhancement was not explored but was suggested to be due to pressure-induced
protein conformational changes or separation of a part of the protein molecule and
subsequent liberation of a second active site. However, there was no indications of
major changes in native and pressure treated onion PPO when analyzed using SDS-
PAGE [92].
Transferases (EC 2)
Polymerase (2.7.7.7)
With the advent of PCR (polymerase chain reaction), DNA polymerases have
become vital in molecular biology [142]. DNA polymerase is the most heat labile
enzyme from the Pyrococcus species [143]. DNA polymerases derived from three
thermophilic microorganisms, Pyrococcus strain ES4, Pyrococcus furiosus, and
34
Thermus aquaticus were stabilized by HP at 111 ˚C, 107 ˚C, and 100 ˚C, respectively
[21]. Half-lives of the three DNA polymerases increased from 5.0, 6.9, and 5.2 min,
respectively, at 3 MPa to 12, 36, and 13 min, respectively at 45 MPa [21]. Pressure
above 45 MPa did not significantly increase the half-life of P. furiosus DNA polymerase,
whereas pressure increase up to 89 MPa did further increase the half-life of DNA
polymerase from Pyrococcus strain ES4 and T. aquaticus [21]. Pressure-induced
stabilization was attributed to pressure effects on thermal unfolding or retardation of
unimolecular inactivation of the unfolded state, and differences between strains is
attributed to differences in the amino acid sequences, which correlate to pressure-
induced stabilization. While application of HP for conducting a PCR assay may not be
currently suitable with today’s technology, any method for stabilizing an enzyme that is
as widely used as polymerase is worthy of further investigation.
Hydrolases (EC 3)
Pectin methylesterase (EC 3.1.1.11)
Pectin methylesterase (PME) catalyzes the demethylesterification (or
demethoxylation) of pectin releasing methanol and protons (creating negatively charged
carboxyl groups) [101, 144] which reduces viscosity and forms low-methoxyl pectin
precipitates resulting in cloud loss of fruit and vegetable juices. This enzyme has been
subject to recent reviews which summarize PME genetic sequencing, elucidation of
three-dimensional structure, the multiple roles of PME in plants, and the existence of
multiple isozymes which differ in their thermal and pressure stability [102].
The rate of recombinant Aspergillus aculeatus PME enzymatic de-esterification
was optimal at 200-300 MPa combined with 45-55 ˚C [99]. Similarly, the highest rate of
PME-catalyzed pectin de-esterification was at 200-300 MPa at 50-55 ˚C [98]. This
35
increase in reaction rate of PME was explained using Le Chatelier’s principle which may
be applicable for de-esterification reactions because charged groups are formed, and
solvation of these charged groups is accompanied by reduced volume resulting from
electrostriction; i.e. the compact alignment of water dipoles owing to the columbic field
of the charged groups [16]. However, Le Chatelier’s principle is only applicable as an
all-encompassing explanation if pressure does not significantly affect PME stability. In
exploration of this caveat to the Le Chatelier’s principle explanation, Fourier transform
IR spectroscopy was used to reveal the pressure stability of β-helices of Aspergillus
aculeatus PME [97]. No significant changes in spectra could be observed up to 1 GPa.
At pressures above 1 GPa, unfolding takes place as indicated by broadening of the
deconvoluted amide I’ band from approximately 1638 cm-1 towards approximately 1635
cm-1 [97]. Pressure stabilization was explained by pressure-induced suppressive effect
on the aggregation of the partially unfolded protein due to the counteracting
hydrophobic forces to a certain extent and by the substantial amount of protein in the β-
helix conformation [97].
Tomato juice PME was activated by pressure above 300 MPa at all temperatures,
and maximal at 300 MPa and 50 ˚C which was almost 1.7 times the control at 0.1 MPa
[103]. This activation was attributed to reversible conformational changes or the enzyme
and/or substrate molecules. In a related study, PME from tomato was quickly
inactivated at 0.1 MPa and 70 ˚C but the inactivation rate constant dramatically
decreased as soon as pressure was raised reaching a minimum between 300 and 600
MPa [94].
36
Extracted and purified carrot PME showed notable pressure resistance (up to 600
MPa) to inactivation in combination with increased catalytic activity with increasing
pressure [101]. The most pronounced activity of carrot PME was observed at 50 ˚C and
500 MPa. Similarly, PME activity in shredded carrots (in situ) was most pronounced at
50 ˚C and 200-400 MPa and 100-400 MPa at 60 ˚C in intact carrots [101]. Similar
results were found with extracted and purified carrot PME at lower pressures (300 MPa)
and higher temperatures (> 50 ˚C) where an antagonistic effect of pressure and heat
was observed [102]. At 60 ˚C, the carrot PME inactivation rate was reduced by greater
than 75% at 300 MPa versus 100 MPa [102]. Since similar results between carrot PME
in shredded carrots and with extracted and purified PME indicate that pressure induced
activation is not related to pressure effects on the substrate (pectin or pectate).
Pressure-treated green peppers showed increased PME activity after treatment
between 100 and 200 MPa for 10 or 20 min compared to the native control [145] and up
to 500 MPa at room temperature [146].
Extracted and purified PME from bananas exhibited the antagonistic effect of
pressure and temperature in the low pressure (≤ 300 MPa) and high-temperature
domain (T ≥ 64 ˚C). Increased pressure resulted in a decrease of the observed
inactivation rate constant [97]. Inactivation rates of orange PME were also slower at 80
˚C and 900 MPa compared to atmospheric pressure and was more pronounced in the
presence of Ca2+ ions (1 M) but less pronounced for the inactivation in an acid medium
(pH 3.7) [100].
While PME is often a target for inactivation in cloudy juices, it is vital for reducing
viscosity of high pectin mixtures and the clarification of cloudless juices such as apple
37
juice. It appears that HHP may be utilized to stabilize PME where needed while
inactivating various other undesirable enzymes during a combined pressure-heat
treatment.
Lipase (EC 3.1.1.3)
Lipases (triacylglycerol acylhydrolases) occur widely in nature where they catalyze
the hydrolysis of esters from glycerol and long-chain fatty acids releasing alcohol and
acid moieties. Since it became accepted that lipases remain enzymatically active in
organic solvents [65] and react in the opposite direction (synthesis of esters), their
application grew and have been the subject of many reviews and studies [49, 147-156].
Lipases now constitute the most important group of biocatalysts for the synthesis of
biopolymers and biodiesel, resolution of racemic mixtures, transesterifications,
regioselective acylation of glycols and menthols, synthesis of peptides, and the
production of enantiopure pharmaceuticals, agrochemicals, and flavor compounds
[153]. Because of their importance to a variety of industries, lipases have been explored
and documented more than any other enzyme at ambient pressure and at HP.
Therefore, lipase is discussed in this review to a greater depth than any other enzyme.
Lipase stability and activity was examined at HP in compressed or supercritical
fluids/gases including carbon dioxide [49, 107-109, 157-167], propane [51, 109, 110,
167], butane [51, 110], sulfur hexafluoride (SCSF5) [51], and mixtures of butane and
propane [51]. Candida Antarctica lipase B (CALB) was effective at synthesizing isoamyl
acetate in SC-CO2 at higher initial reaction rates when compared to n-hexane while
maintaining activity from 8 to 30 MPa [161]. These results were explained as being due
to improved diffusivity of the reactants in the medium. CALB was also successfully used
as a catalyst to synthesize butyl butyrate in SC-CO2 [108]. All supercritical conditions
38
assayed enhanced activity 84-fold with respect to synthesis in organic solvents while
maintaining stability showing a 360 cycle half-life. Best results were achieved at 60 ˚C
and 8 MPa and were explained as improved micro-environments around the enzyme
[108].
The apparent kinetics of immobilized CALB synthesis of isoamyl acetate at HHP in
hexane has also been examined. Activity of CALB increased by 110% at low pressure
versus a 239% increase at 350 MPa when the temperature was increased from 40 to 80
°C. Increasing pressure up to 350 MPa increased lipase activity, while pressures
greater than 350 MPa maintained or decreased lipase activity. ΔV≠ appeared negative
between ambient pressure and 200 MPa in contrast to a positive ΔV≠ between 300 and
600 MPa. Besides increasing activity, HHP also reduced thermal inactivation of CALB
by up to 152% after 4 h at 80 °C and 400 MPa when compared to incubations at low
pressure [168]. Lipase activity at 63.5 and 80 °C at 400 MPa was greater (from about 20
to 96% increase) than at low pressure [168].
Rhizomucor miehei lipase was used in the esterification of lauryl oleate from oleic
acid and 1-dodecanol in a batch stirred reactor using dense CO2 as a reaction medium
where the catalytic efficiency increased up to 10 MPa and was attributed to either
substrate-solvent clustering, stabilization effect of SC-CO2 treatment, or to the
stabilization of lipase in the “open” form by hydrophobic interactions [104]. HHP in an
aqueous medium has also been shown to improve lipase from Rhizomucor miehei. At
denaturing temperatures (50, 55, and 60 ˚C), application of 50 to 350 MPa protected the
lipase. This protective effect increased with temperature [106]. Similarly, the protective
effect of pressure against thermal inactivation (50 and 55 ˚C) was observed for
39
Rhizomucor miehei lipase at 50 – 450 MPa [105]. Conformational studies using
fluorescence spectroscopy suggested that the conformational changes induced by
pressure were different from those induced by temperature [169]. Noel and Combes
[169] also concluded that Rhizomucor miehei lipase has a high stability under pressure
as it represents a slight change in volume (0.2%) in comparison to the initial volume of
the native protein. Conversely, Osorio and others [170] found for lipase from
Thermomyces lanuginose increasing pressure improved selectivity while it linearly
decreased stability.
Catalytic efficiency of Pseudomonas cepacea lipase transesterification of 1-
phenylethanol and vinyl acetate in SC-CO2 increased up to 15 MPa [55] and was more
thermostable in supercritical propane than in water (optimum temperature increased
from 36.8 ˚C in water to 49.8 ˚C in propane) [167]. This was hypothesized to be a
consequence of protein structural and conformational rigidity in propane. In the same
study lipases from Pseudomonas fluorescences, Rhizpous javanicus, Rhizopus niveus,
and porcine pancreas were stable in SC-CO2 and near-critical propane as activity
remained constant after 24 h at 30 MPa and 40 ˚C. Recently, activity of lipase from
porcine pancreas, Candida antarctica, Aspergillus oryzae, Candida cylindracea,
Penicillium roqueforti, Aspergillus niger, Rhizopus arrhizums, Mucor miehei, and
Pseudomonas cepacia was increased after reacting at 40 ˚C and 15 MPa in SC-CO2
[171]. The most remarkable increase in activity was from Rhizopus arrhizums lipase
where activity increased 50 fold [171].
Lipase from Candida cylindracea used for the esterification between n-valeric and
citronellol was shown to have a reaction rate dependence on pressure [165] which
40
increased significantly until reaching a maximum at 7.55 MPa near the critical point of
SC-CO2 [165]. Increased activity was explained by interactions between carbon dioxide
and enzyme molecules inducing drastic conformational changes of the enzyme, causing
active sites to emerge and catalyze the stereoselective synthesis [165].
Crystallographic and molecular-modeling studies of CALB determined that lipase
belongs to the α/β hydrolase fold family with a catalytic triad consisting of Ser, His, and
Asp/Glu [172]. Early X-ray diffraction data suggests that a lipase’s helical part of the α-
helix near the active site forms a “lid” that rotates almost 90˚, from lying flat on the
surface to extending nearly perpendicular to it on rearrangement to the open
conformation [173]. This “lid” is shifted aside thus exposing the active site and
generating the “active” form of lipase. This mechanism was suggested [104] for lipase
(lipozyme RM-IM) activation at pressure close to 10 MPa in CO2. Knez and others [104]
explained in such a condition the “lid” is moved away (rolls back) and the hydrophobic
CO2 molecules stick out around the active site, following the opening of the lid,
unblocking the entrance of the tunnel. Uppenberg and others [172] suggested that the
α-helix (α5) can be stabilized by hydrophobic molecules at the entrance of the active
site pocket.
Recent studies conducted in aqueous media have concluded that in contrast to
most lipases, CALB may not have a “lid” blocking access to the active site and shows
no interfacial activation [68] as compared to Candida antarctica lipase A (CALA) which
does possess the characteristic “lid” structure and shows interfacial activation [174].
Furthermore, flexibility of CALB is reduced in organic solvents, and is limited to: (1) a
short α-helix which form the entrance to the active site, (2) three surface loops, (3) the
41
medium binding pocket for secondary alcohols, (4) the acyl binding pocket, and (5) the
large binding pocket for secondary alcohols [68]. Flexibility limited to these five
elements vital to catalysis may offer possible explanation for relatively HP stability, while
still allowing modification of activity. Since lipases are widely used in high value product
(fine flavors, pharmaceuticals, etc.) biosynthesis, the use of HP technologies may be
uniquely suitable due to cost effectiveness associated with these products.
Acetylcholinesterase (EC. 3.1.1.7)
Acetylcholinesterase is indispensible in synaptic transmission by catalyzing
hydrolysis of acetylcholine and plays a role in stress response, degenerative diseases,
and neural development in humans [175]. Acetylcholinesterase 7.4S was more active at
pressures up to approximately 14 MPa when compared to 0.1 MPa [112]. Pressure
induced stability appeared to be related to the 7.4S enzyme having a large volume
expansion accompanying the activity loss apparently retarded by application of
moderate to low pressure. This enzyme is the only pressure-enhanced enzyme native
to human physiology neural synaptic system. Acetylcholinesterase is widely used in
various biosensors mainly for the detection of pesticides but also for detection of metal
cat ions, inorganic metals, as well as other organic compounds [176]. Therefore it may
be a suitable candidate for a pressure stable biosensor used in HP environments such
as deep-sea exploration and deep underground oil, natural gas, and water drilling.
Polygalacturonase (EC 3.2.1.15)
Polygalacturonase (PG) catalyzes the α-1,4-glycosidic bonds of the product of
PME catalyzed pectin de-esterification. This depolymerization leads to a drastic
decrease in viscosity of various fruit and vegetable juices. Unlike PME, increases in
pressure and temperature can accelerate the inactivation rate of PG [94]. However, a
42
pressure resistant PG fraction from tomato was not affected by prolonged pressurization
up to 600 MPa at 50 ˚C [113]. Furthermore, PG activity increased up to optimal
pressure (100-200 MPa) depending on the temperature [177]. Verlent and others [177]
found that PG catalyzed hydrolysis of pectin in the presence of tomato PME remains
constant with increasing pressure at 50 ˚C which is in contrast to earlier work by the
same group [178, 179] where a shift in optimal temperature to lower values was
observed with increasing pressure. The relationship between PG activity with or without
PME needs further exploration; however it is clear the HP can be utilized to modulate
activities to achieve desired processing conditions such as increasing PG activity to
reduce fruit or vegetable juice viscosity.
α-Amylase (EC. 3.2.1.1)
α-Amylase catalyzes the hydrolysis of 1,4-α-D-glucosidic linkages in
polysaccharides containing three or more 1,4-α-linked D-glucose units in random order
[114] and used mainly to degrade starch to low molecular weight dextrins in the
production of sugar syrups [180] as well as for the preparation process of alcoholic
beverages such as beer and whisky [114]. Studies from the 1950s described by Laidler
[181] identified a “salivary amylase” and a “pancreatic amylase” which both had ΔV≠ = -
22 cm3 mol-1 and -28cm3 mol-1 respectively. More recently, α-amylase from barley malt
was stabilized against thermal inactivation up to 200 MPa with maximum substrate
cleavage at 152 MPa and 64 ˚C with 25% higher yield as compared to the maximum at
ambient pressure and 59 ˚C [114]. The optimum conditions are explained by the
superposition of pressure induced thermal stabilization of the enzyme and enhanced
substrate conversion by temperature. Treatment of α-amylase with SC-CO2 and 0.1%
43
water at 35 ˚C and 20 MPa for 1 h resulted in residual activity of 105% compared to
prior to treatment [182].
β-Amylase (EC. 3.2.1.2)
β-Amylase hydrolyzes the α-1,4-glucosidic linkages of starch from the non-
reducing ends. This reaction is utilized in the food and beverage industry for the
preparation of fermented foods or maltose production as a precursor for alcoholic
beverages. The effects of HP on the flexibility of subgroups within β-amylase have been
observed by monitoring intensity changes in the near UV spectrum and with circular
dichroism [183]. β-amylase activity from barley malt was strongly affected by HP and
temperature treatment [115]. Highest depolymerization of starch rate was found at 100
MPa and 62 ˚C, yielding 15% more compared to optimum conditions at ambient
pressure [115]. The shift in temperature optimum was attributed to the stabilization of
the enzyme against thermal inactivation. Like α-amylase, HP may be utilized to improve
β-amylase catalysis for use in the production of sugar syrups or alcoholic products.
β-Glucanase (EC. 3.2.1.2)
β-Glucanase activity in malt is crucial for the brewing process because of its effect
on beer filtration. β-Glucanase depolymerizes β-glucans which increase beer viscosity
by thus reducing filterability [184, 185]. β-Glucanases are synthesized during
germination but are inactivated at temperatures above 50 ˚C during the malting and
mashing processes. Pressure (400 MPa) significantly stabilized this enzyme against
thermal inactivation [116]. However, increasing pressure also decreased activity up to
600 MPa [116]. Counteracting effects of stabilization and reduced activation resulted in
maximum conditions at 215 MPa and 55 ˚C which yielded approximately 2/3 higher
degradation of β-glucan after 20 min as compared to the maximum at 0.1 MPa at 45 ˚C
44
[116]. No discussion was provided with regards to substrate stabilization, or pressure
effects on substrate. It is clear that high hydrostatic pressure along with elevated
temperature can be utilized to improve β-glucanase activity for depolymerizing β-
glucans.
Glucoamylase (EC. 3.2.1.3)
Glucoamylase is a multidomain exo-glycosidase that catalyses the hydrolysis of α-
1,4 and α-1,6 glucosidic linkages of starch and related polysaccharides to release β-D-
glucose from the non-reducing ends and is used in the production of spirits and glucose
syrups from starch [117]. Two isoforms of glucoamylase (GA1 and GA2) from
Aspergillus niger were studied for their response to pressure temperature treatments.
The pressure liable form of glucoamylase (GA2) was inactivated above 850 MPa
whereas the stable (GA1) isoform was slow to inactivate up to 1400 MPa at 50 ˚C [117].
Pressure stabilized the enzymes against thermal inactivation at 400 MPa for GA2 and at
550 MPa for GA1 [117]. Since elevated pressure contributed to delayed enzyme-
substrate interaction up to 600 MPa, the maximum production of glucose by maltose
cleavage was observed at approximately 84 ˚C and 318 MPa after 30 min [117]. β-
Glucoamylase from barley malt exhibited a maximum depolymerization rate at 215 MPa
and 55 ˚C which yielded approximately 2/3 higher degradation of β-glucan after 20 min
as compared to the maximum at 0.1 MPa and 45 ˚C [116]. Activity also increased 102
and 105% after treatment with SC-CO2 and SC-CO2 + 0.1 wt% water respectively at 35
˚C and 20 MPa for 1 h compared to prior to treatment [182]. Like α-amylase, β-amylase,
and β-glucanase discussed earlier, glucoamylase is widely used in the brewing industry
and shows a clear activity and stability enhancement at elevated pressures. The
45
evidence of pressure enhancement of these four enzymes vital for beer and spirit
production are examples of the potential improvement of industrial processes with HP.
Lysozyme (EC. 3.2.1.17)
Lysozyme is commonly found in nature and is primarily from egg albumin.
Lysozyme hydrolyzes the β-1,4 glycosidic bond between the N-acetylmuranimic acid
and the N-acetyl-D-glucosamine of peptidoglycan, which is the major component of
gram-positive bacteria cell walls [186]. Lysozyme is relatively low-priced as compared to
other antimicrobial agents such as nisin [187], is classified as generally recognized as
safe (GRAS), and is effective as a food preservative by inhibition of pathogenic and
spoilage bacteria [186, 188-191]. Lysozyme activity is relatively stable below 200 MPa
while above 200 MPa some enzymatic activity is lost but antimicrobial activity was not
reduced [186]. Iuccie and others [192] also found that lysozyme treated at 100 MPa had
increased antimicrobial activity resulting in approximately two logarithmic reductions in
microbial death. The increase in antimicrobial activity was attributed to a direct effect of
pressure on the integrity of cell walls or outer membranes of the microbes, a
consequent increased penetration of enzymes through the damaged walls or
membranes, and indirect effects on the processes of the antimicrobial properties of
lysozyme [192]. While pressure increased the antimicrobial activity of lysozyme, it may
be a synergistic or additive effect and not purely attributed to increased enzymatic
activity. Although pressure effects on lysozyme activity above 200 MPa remain unclear,
current evidence suggests that pressures below 200 MPa may aid in the action of this
widely used, effective, and relatively inexpensive antimicrobial enzyme.
46
β-Glucosidase (EC. 3.2.1.21)
β-Glucosidase catalyzes the hydrolysis of aryl and alkyl β-D-glucosides and are
involved in key metabolic events and growth related response in plants [193]. This
enzyme is involved in the liberation of volatile aglycones from non-volatile glucosides
[194] and is important to for subsequent flavor release [88]. In red raspberries, HPT at
400 MPa increased activity 2 % while in strawberries HPT of 400 MPa increased activity
76% [88]. β-glucosidase from Sulfolobus solfactaricus was also activated by pressure
between 0.1 and 250 MPa with maximal activity at 125 MPa and has a half-life of 91 h
at 60 ˚C and 250 MPa. Conversely almond β-glucosidase was rapidly inactivated by
pressure up to 150 MPa [195]. HP activation may be helpful in strawberry or raspberry
processing where pressure is used to inactivate some unwanted enzymes while
activating others that contribute to flavor development.
β-Galactosidase (EC. 3.2.1.23)
β-Galactosidases are widely used in the food industry to hydrolyze lactose into
galactose and glucose [118]. Also, the transgalactosidase activity of β-galactosidases
can be useful in synthesis of glyconjugates for food and pharmaceutical applications
[196, 197]. β-galactosidases from Aspergillus oryzae, Kluyveromyces lactis, and
Escherichia coli were investigated for their increased thermostability under HP. After 1 h
incubation at 25 ˚C residual activity did not significantly decrease for β-galactosidase
from A. oryzae below 450 MPa, below 300 MPa from E. coli, and below 200 MPa from
K. lactis [118]. For the three enzymes tested, moderate pressures protected the enzyme
against thermal inactivation. Residual activity of E. coli β-galactosidase increased from
60% at 0.1 MPa to 80% at 100 MPa and 55 ˚C [118]. Residual activity of K. lactis β-
galactosidase increased 5-fold at 100 MPa versus at 0.1 MPa and 45 ˚C [118]. Most
47
interestingly, residual activity of A. oryzae β-galactosidase increased from complete
inactivation at 55 ˚C and 0.1 MPa to near 100% residual activity at 250 MPa for a 1 h
incubation [118]. β-galactosidase from E. coli had no decrease in activity below 250
MPa [198] and at 250 MPa the half life at 55 ˚C was 32 h versus 1.5 h at 0.1 MPa [199].
While application of HP to β-galactosidase in the food industry may be advantageous,
as with many enzymes the application of HP for pharmaceutical synthesis of
compounds such as glyconjugates may be more economically viable.
Invertase (EC. 3.2.1.26)
Invertase (β-D-fructofuranosidase) is widely used in the food industry for its
hydrolytic activity on sucrose for the production of invert sugar (mixture of glucose,
fructose, and unhydrolyzed sucrose) [200]. Pressure induced conformation changes
were determined using Raman Spectroscopy [201] and fluorescence spectroscopy
[202] where conformational changes induced by pressure and temperature were
different. HP caused an increase in low-wave number scatter in solution and to a shift of
the amide I bands lower while thermal denaturation showed no such modifications in
spectra [201]. Likewise, thermal treatment of invertase caused the fluorescence of
tyrosine and tryptophan to decrease slowly while HPT caused these aromatic residues
to become more exposed causing increased fluorescence [202]. These differences
were hypothesized to be due to HP and temperature exerting opposing effects on weak
interactions (hydrogen bonds, ionic and hydrophobic interactions) leading to different
denaturation mechanisms [201] and may explain the antagonistic effects of pressure
and temperature for invertase pressure induced stabilization. Saccharomyces
cerevisiae invertase half-life increased at 60 ˚C from 50 to 200 MPa [106]. Furthermore,
native and immobilized invertase have ΔV≠ = -7.3 cm3 ∙mol-1 [203] and ΔV≠ = -29 cm3 ∙
48
mol-1 [204] respectively. Conversely, invertase can be readily inactivated by pressure
depending on the specific temperature-pressure combination [202, 205].
Naringinase (EC. 3.2.1.40)
Naringinase is used to reduce bitterness in grapefruit juice by hydrolyzing naringin
(a flavonone glycoside and primary bitter component in grapefruit juice) to naringenin,
which is tasteless. In a model solution, naringinase activity increased by 72% at 200
MPa and 54 ˚C versus only a 35% reduction at 0.1 MPa [122]. These results are in
agreement with earlier findings where maximum naringinase activity was between 30
and 40 ˚C and approximately 160 MPa with a ΔV≠ = -9 to -15.0 cm3 mol-1 [119-121]
depending on immobilization technique and other reaction conditions. The HP induced
activation of naringinase makes it suitable for grapefruit juice processing as modified
conditions can optimize naringinase activity while simultaneously inactivating
undesirable pressure-labile microorganisms.
Myrosinase (EC. 3.2.3.1)
Glucosinolate hydrolysis products in broccoli catalyzed by myrosinase such as
sulforaphane are thought to have beneficial health effects. Therefore, a heat and
pressure treatment that results in stabilized myrosinase could be advantageous [124].
Inactivation rate constants decreased up to a maximum around 350 MPa at 35 ˚C.
These results were later substantiated when thermal treatment of 60 ˚C reduced activity
by 97% at 0.1 MPa versus 75% at 100 MPa [124]. The activation energy of myrosinase
inactivation was highest at 200 MPa, the pressure at which the antagonistic effect was
most pronounced [124]. This antagonistic effect was not observed with a second form of
myrosinase for which inactivation rates continually increased with increased pressure
[123]. The application of HP may effectively improve the inactivation of deleterious
49
enzymes and microbes while simultaneously increasing or preserving the activity of
beneficial enzymes such as myrosinase. Although the relationship between myrosinase
activity and pressure is not fully elucidated, it is clear that application of elevated
pressure may be a useful tool in the enhancement of health benefits of processed
broccoli.
α-Chymotrypsin (EC. 3.4.21.1)
α-Chymotrypsin (CT) is a proteolytic enzyme that facilitates the hydrolysis of
peptide bonds and is used to aid protein digestion. It is a serine protease with the
characteristic three amino acid active site known as the catalytic triad. Stability of α-
chymotrypsin at HP was investigated in the 1940s [127]. While no pressure-induced
activation was noted, induced stabilization was reported up to 760 MPa. Pressure
effects on CT activity and stability were explored again in the 1980s by Taniguchi and
Suzuki [128] and in more depth in the mid 1990s by Mozhaev and others [41, 125].
Taniguchi and Suzuki found that increasing pressure increased CT hydrolysis of p-
nitrophenyl acetate from 10 to 65 ˚C with maximal activity at 45 ˚C and 200 MPa [128]
and pressure activation was more pronounced as temperature increased. Similarly,
Mozhaev and others found that an increase in pressure at 20 ˚C resulted in a 6.5-fold
increase in activity at 470 MPa versus 0.1 MPa [125]. The acceleration effect became
more pronounced at high temperatures as activity at 50 ˚C and 360 MPa was 30-fold
higher than activity at 0.1 MPa and 20 ˚C [125]. High pressure also increased stability of
CT. CT is readily inactivated (less than 5 min half-life) at 0.1 MPa; while at 180 MPa CT
remains active for 30 min [125]. Stability and activity of CT was also improved by
pressure in organic media when Mozhaev and others [126] obtained ΔV≠ = -13 ± 2 cm3
mol-1 while maintaining activity up to 200 MPa. This was explained as being due to a
50
transitional conformation between 100 and 150 MPa that renders the enzyme more
active. Raman spectroscopy was used to explore pressure-induced structural changes
and found only slight changes up to 200 MPa that were attributed to the salt bridge
between Asp-194 and Ile-16 [206]. While many enzymes native to muscle tissue are a
target for inactivation by HP [207], the pressure-induced stabilization or activation of α-
chymotrypsin may be useful in modifying the functional and organoleptic properties of a
wide variety of processed meat products.
Thermolysin (EC. 3.4.24.27)
Thermolysin is used in the production of a precursor for a synthetic sweetener and
may be suitable for the production of various peptides through the condensation of
amino acids [208]. Thermolysin hydrolysis of β-lactoglobulin (BLG) rate increased by a
factor of 22 from 0.1 to 200 MPa before irreversible conformational changes occurred at
or above 300 MPa [129]. Similarly, BLG digestion by thermolysin increased from 19.4 to
25.0% at 200 MPa versus at 0.1 MPa [208]. In the same study thermolysin catalysis
was accelerated by increasing pressure on nonspecific digestion of proteins from
various origins. These proteins included, alcohol dehydrogenase (18.1% versus 45.3%),
hemoglobin (13.0% versus 34.6%), bovine serum albumin (0.19% versus 0.23%), and
myoglobin (12.0% versus 15.0%) at 0.1 MPa and 200 MPa respectively [208].
Increased reaction rate was attributed to pressure effects on enzymatic activation as
well as protein substrate partial unfolding allowing greater catalytic activity on the
protein substrate. This combined pressure effect is dually useful when conducting
enzymatic catalyzed synthesis or hydrolysis reactions because pressure can act as a
denaturation-inducing agent. This pressure effect on substrate denaturation was termed
“reagent-less denaturant” by Kunugi [208].
51
A thermostable neutral thermolysin from Bacillus thermoproteolyticus was
compared to a non-thermostable neutral thermolysin from Bacillus subtilis [209]. The
application of 100 MPa resulted in over 13 times increase in reaction rate for the
thermostable enzyme versus 3.8 times increase for the non-thermostable enzyme [209].
Also, thermolysin catalyzed hydrolysis of a dipeptide substrate (FA-Gly-Leu-NH2) had a
ΔV≠ = -30.2 cm3 mol-1 [210]. Thermolysin from Bacillus thermoproteolyticus was also
shown to have ΔV≠ = -52 ± 4 cm3 mol-1 and up to a 40-fold reaction acceleration at 100
MPa and 40 ˚C for hydrolysis of the low molecular mass substrate 3(2-furylacrylolyl)-
glycyl-L-leucine amide [211]. HP also increased residual activity by 101 and 102% after
treatment with SC-CO2 and SC-CO2 + 0.1% water at 35 ˚C and 20 MPa for 1 h resulted
compared to before treatment [182]. Similarly to lipase, thermolysin is used in high-
value product (synthetic sweetener and peptide) biosynthesis; and therefore, use of HP
technologies may be suitable due to the cost effectiveness associated with these
products.
Pepsin (EC. 3.4.23.1)
Like thermolysin, pepsin is used as a catalyst in the production of a precursor for a
synthetic sweetener and may be suitable for the production of various peptides through
the condensation of amino acids [208]. The hydrolysis of BLG with pepsin was studied
between 0.1 and 350 MPa. Increased pressure showed a significant increase in
cleavage rates [129]. Pepsin was unable to hydrolyze BLG at 0.1 MPa versus total
hydrolysis of all the BLG substrate in less than 40 min at 300 MPa [129]. The BLG
peptic hydrolysis rate increased 270-fold between 0.1 and 300 MPa. Like lipase and
thermolysin, pepsin can be used in high-value product biosynthesis. Therefore the use
52
of HP technologies may be suitable due to cost effectiveness associated with these
products.
Unidentified protease
Proteases traditionally are applicable for the cleavage or digestion of proteins,
which is particularly useful in the food or pharmaceutical industry. The properties of an
unidentified and un-named protease from a hyperthermophilic barophilic
Methanococcus jannashii, an extremely thermophilic deep-sea methanogen found at a
deep-sea hydrothermal vent, have been explored. The activity and stability of the
partially purified enzyme increased with pressure; raising the pressure increased the
reaction rate 3.4-fold and the thermostability 2.7-fold at 50 MPa at 125 ˚C with a
corresponding negative activation volume of -106 cm3 mol-1 [20] compared to 0.1 MPa.
The barophilic behavior of this protease is somewhat expected in view of the unusual
barophilicity exhibited by M. jannashii [212], as well as other enzymes from this
organism such as hydrogenases discussed earlier [86, 87].
Pyrophosphatase (3.6.1.1)
Pyrophosphatases are acid anhydride hydrolases that act upon diphosphate
bonds and are used in DNA polymerization reactions for in vitro RNA synthesis
reactions and for pyrophosphate removal which is from biosynthetic reactions that utilize
ATP [213, 214]. Inorganic pyrophosphatase from yeast was partially stabilized against
thermal inactivation by the addition of trehalose and glycerol [215]. Partially purified
pyrophosphatase from Bacillus stearothermophilus demonstrated increased activity at
90 ˚C from 10 to 100 MPa with optimal activity at 70 MPa [130]. No activity could be
demonstrated at 100 ˚C at 0.1 MPa while at 105 ˚C and 103 to 190 MPa activity
increased up to 320% compared to 0.1 MPa [130]. Activation was explained by
53
pressure counteracting the molecular volume increase which results from elevated
temperatures. While this explanation is over-simplified, for the time of publication it was
considered adequate. Like polymerase, the application of HP for conducting a DNA
analysis may not be currently suitable with today’s technology, although any method for
stabilizing a widely used enzyme is worthy of further investigation.
Lyases (EC 4)
Aspartase (4.3.1.1)
Aspartase (L-aspartate ammonia-lyase) catalyzes the reversible deamination of
the amino acid L-aspartic acid producing fumaric acid and ammonium ion [214, 216]. It
was used to produce L-aspartic acid on a large scale [217, 218]. Aspartase of
Escherichia coli was shown to be activated by pressure in the early 1960s as activity
increased from 0.1 MPa to 100 MPa at 50 ˚C and from 0.1 MPa to 60 MPa at 53 ˚C and
56 ˚C [131]. It was suggested that the application of pressure may increase the
incidence of substrate-active site collision as well as prevent enzyme unfolding. Like
other early studies, this explanation was adequate for the time of publication but is
understood to be an oversimplification.
Remaining Challenges
Although the effect of pressure on the stability and rates of reaction for many
enzymes has been researched, there is still a lack of experimental data for the majority
of known enzymes. Also, the effect of HP on enzyme structure is scarce because there
are very few laboratories equipped with HP optical cells coupled to the instrumentation
necessary for such studies. Currently, most methods require introducing enzyme to
substrate then applying incubation conditions for a given time interval. After a given
time, the enzyme reaction mixture is removed from the incubator and assayed, and
54
repeating this procedure at time intervals allows pseudo-apparent kinetic
measurements. Although such efforts as precisely controlling temperature and enzyme
to substrate ratios among other reaction parameters can effectively slow the reaction to
give adequate apparent kinetic measurements, they must compensate for adiabatic
heating and cooling and the pressurization and depressurization transient time. For
these reasons, future studies are needed to develop in-situ kinetic measurements at HP
with precise control of other reaction parameters such as temperature. Likewise, in-situ
studies need to be conducted to fully elucidate quaternary, tertiary, and even secondary
structural changes during pressure changes, at isobaric conditions, and at various
combinations of temperature and pressure. These studies will allow greater
understanding of enzymatic changes at elevated pressures which may allow for better
utilization and optimization of reaction conditions.
Despite its advantages described here, the application of HP for enzymatic
reactions may not always be practical due to the high cost of HP systems, lack of
appreciable effects, or advancements in alternative enzyme enhancement technologies.
However HP has great potential and is only beginning to be explored in the field of
enhancing enzyme systems.
Specific Objectives
The central hypothesis of this research is that high pressure can be used to
increase lipase activity and stability. The overall objective of this research is to
document the effects of high hydrostatic pressure on free and immobilized lipase
catalyzed isoamyl acetate synthesis in selected solvents. The first specific objective is
to determine the stabilization and activation effects of HHP on immobilized lipase in
hexane. The working hypothesis is that high pressure will increase immobilized lipase
55
activity and stability in hexane. This objective will be achieved by determination of
several parameters; including ΔV‡, Ea, Vmax, and KM while also observing the effects of
HHP on the immobilization support. The second specific objective is to determine the
effect of HHP on immobilized and free lipase catalyzed synthesis of isoamyl acetate in
an ionic liquid-alcoholic biphasic mixture. The working hypothesis of this specific
objective is that the combination of using IL-alcohol biphasic mixtures and HHP will
provide a new method of increasing the reaction rate of free and immobilized lipase. To
achieve this second specific objective it is necessary to determine the ΔV‡, Ea. The last
specific objective is to continuously monitor in situ conformational studies of free lipase
as it is subjected to thermal and HHP treatment. The working hypothesis of the third
specific objective is that conformational changes occur within the lipase at HHP and are
different depending on the temperature-pressure combination. This specific objective
will be achieved by recording fluorescence intensity changes induced by changes in the
tertiary structure of the lipase (mainly tryptophan).
56
Figure 1-1. Theoretical generic elliptical pressure versus temperature diagram with native and denatured protein regions inside and outside of the ellipse respectively, separated by a zone of reversible denaturation.
57
CHAPTER 2 HIGH HYDROSTATIC PRESSURE INCREASED STABILITY AND ACTIVITY OF
IMMOBIILZED LIPASE IN HEXANE
Introduction
Enzymes important to high value product synthesis are often expensive and
unstable above 40 °C. Various strategies have been employed to enhance enzyme
stability including genetic engineering, immobilization, and operating in non-aqueous
media. Isoamyl acetate has been widely used (74,000 kg/year) as a flavor or aroma
ingredient in food, cosmetic, and pharmaceutical industries because of its characteristic
banana flavor [219] and ability to be considered “natural” [220]. Because conventional
flavor generation from plant materials or production via microbial fermentation requires
several costly steps an alternative enzymatic method using lipases has become the
focus of many studies [38, 42, 45, 52, 67, 161, 221, 222]. Lipases are widely used in
industrial applications because of their high enantioselectivity, wide range of substrates,
thermal stability, and stability in organic solvents [223]. Isoamyl acetate esterification
catalyzed by lipases from various sources has been studied in a wide variety of solvents
[38, 52, 161], kinetic studies have proposed a Ping-Pong Bi-Bi mechanism [221], and
operating conditions such as acyl donor, type of lipase, and temperature have been
optimized [38]. However, the application of high hydrostatic pressure (HHP) as a
reaction parameter has not been explored in hexane.
While HHP is effective at inactivating various deleterious enzymes [8-14], its
effects on enzyme stabilization and activation have been documented relatively little
[15-19]. HHP has been shown to stabilize or activate chymotrypsin [125], naringinase
[120, 121], polyphenol oxidase [13], pectin methylesterase [13, 97, 99], and more
extensively lipases in dense gases and solvent free systems [50, 104, 109, 110, 159,
58
161, 167] among many others. No work to date has focused on investigating HHP
enhanced stability or increased activity of lipase catalyzed synthesis of isoamyl acetate
in an organic solvent.
Pressure and heat are generally thought to be antagonistic factors in molecular
terms (from the principle of microscopic ordering, an increase in pressure at constant
temperature leads to an ordering of molecules or a decrease in the entropy of the
system) and with regards to enzyme conformation [17-19, 28]. This antagonistic
relationship results in an elliptical pressure vs. temperature diagram with native and
denatured protein regions inside and outside of the ellipse, respectively [17]. During the
pressure and temperature come-up time the enzyme may undergo irreversible
denaturation that results in a decrease in activity. While these antagonistic effects have
been previously explored and discussed [17-19, 28] no work to date has compared the
different effects of applying HHP first then heating, heating first then applying HHP, or
attempted to apply HHP and heat simultaneously and assessed the effects on rate
constant and activation energy, in particular for lipase-catalyzed synthesis of isoamyl
acetate in organic solvent.
Operating at HHP offers other less complex advantages over conventional
synthesis at ambient pressures. For example, Candida antarctica lipase B (CALB) is a
relatively heat-tolerant enzyme that is active up to 100 °C [38]. Furthermore, several
other extremely heat-tolerant (stable up to 150 °C) enzymes have been discovered and
may have a potential application in biocatalysis in organic media [22-24]. However, the
boiling point of most organic solvents is well below 100 °C. For example hexane boils at
67.8 °C (at 0.1 MPa) which restricts studies in hexane to be explored below 65 °C. As
59
pressure is raised the boiling point of organic solvents also increases allowing studies to
examine activity above conventional temperatures at low pressure [25]. The ability to
operate with organic or volatile solvents at temperatures above their conventional
boiling point is a significant yet often overlooked advantage of HHP.
The cost of high pressure processing (HPP) has decreased over the last decade
and become more widely implemented particularly in the food industry. In 2007 there
were about 120 HPP industrial installations operating worldwide [26] with 80 % of their
equipment installed since 2000. HPP food has become a two billion dollar global market
and is expected to comprise 450 million pounds/year in 2008 [27]. As demand for HPP
equipment grows, innovation is expected to continue to reduce capital and operating
costs [26]. Although HPP of bulk foods is currently more widespread, the much higher
profit-margin sector of enzyme catalyzed flavor synthesis may have greater potential for
adopting HPP.
The objective of this research was to characterize the effects of HHP and
temperature on lipase activity and stability during the synthesis of isoamyl acetate in
hexane.
Materials and Methods
Materials
Lipase (Novozyme 435® E.C. 3.1.1.3) from Candida antarctica lipase B (CALB)
expressed in Aspergillus oryzae immobilized on a macro porous acrylic resin (13,100
PLU/g) was obtained from Sigma Aldrich (St. Louis, MO USA). Isoamyl alcohol, glacial
acetic acid, and HPLC grade hexane were obtained from Fisher Scientific (Pittsburg, PA
USA). All solvents and substrates were held at -10 °C or on ice while preparing for
assay. Reaction vials were made using 3-mL syringes with Luer-Lock™ tips (BD Franklin
60
Lakes, NJ USA) which allowed substrate insertion with an opposing plunger while
preventing solvent, substrate, or enzyme leaching during pressurization.
The HHP system consisted of a high pressure reactor (model U111), a high
pressure micropump (model MP5), and a pump controller (MP5 micropump control unit)
all from Unipress Equipment (Warsaw, Poland). The reactor was temperature-controlled
with a water jacket alternatively fed by two water baths (Isotemp 3016D); one cooling (5
or 10 °C) and another heating (25 to 80 °C ± 0.1 °C) from Fisher Scientific and
controlled by an array of pinch valves. Computer programs written in LabVIEW and a
data acquisition board (DAQ Card 6062E) with a signal conditioner (model SC-2345)
from National Instruments (Austin, TX USA) were used to collect temperature and
pressure data and to control the heating/cooling valve array. The HHP system is
depicted in Fig. 2-1 and shown in Appendix 1. Stirring inside the reaction vial was
initiated by a magnetic stir-bar inside the reaction vessel and controlled by external
spinning neodymium magnets on an AC motor type NS1-12 (Bodine Electric Company,
Chicago, IL USA). Reaction progress was monitored using GC-FID 5890 (HP, Palo
Alto, CA USA) with a ZB-5 column (30 m length × .53 mm ID × 1.5 μm thickness) at a
gradient temperature from 50 °C to 90 °C at 5 °C min-1. Injector temperature was held
at 200 °C and FID detector at 250 °C. The scanning electron microscope (SEM) was a
Hitachi model S-530 (Tokyo Japan). Samples were coated using a Ladd (Williston, VT
USA) sputter coater.
Methods
Effect of HHP on lipase stability
Enzyme was weighed (10 mg or ~128 Propyl Laureate Units) into the reaction vial.
One milliliter of hexane and a miniature stir bar were added to the enzyme. The reaction
61
vial plunger was moved into position to eliminate air bubbles then sealed with a
Leur-lock™ plug. The reaction vial was then placed in the high pressure reaction
chamber being held at 10 °C. Polydimethylsiloxane silicone liquid (Accumetric, Inc.,
Elizabethtown, KY USA) was added as hydraulic fluid to fill the reactor. The reactor was
sealed and pressurized. After pressure reached the set-point, temperature was adjusted
to 80 °C. Incubations were held at pressures from 10 to 700 MPa for 4 h. Upon
completion of incubation, the temperature was returned to 10 °C, and the reactor was
depressurized and opened. The reaction vial was withdrawn. Lipase activity was
determined by monitoring the reaction progress of the esterification of isoamyl alcohol
and acetic acid to form isoamyl acetate as previously described [38, 221] and shown in
equation 2-1.
Isoamyl Alcohol
CH3
OH
CH3
CH3
O
OH
CH3
O
O
CH3
CH3OH2+ +
Lipase
Acetic Acid Isoamyl Acetate(2-1)
The esterification reaction was initiated by addition of 1 mL 0.12 M isoamyl alcohol
in hexane and 1 mL of 0.12 M acetic acid in hexane combined to make 0.06 M
substrate solution into the reaction vial though the luer-lok™. The reaction mixture was
incubated at 10 °C and stirred continuously. A 1-μL aliquot was drawn for GC-FID
analysis every 10 min. The apparent initial rate was determined by linear regression of
the progress curve in the linear range (time ≤ 30 min). Peak identification was
determined using pure standards. Reaction stoichiometry has been recently reviewed
and confirmed [38, 42, 221], which allowed kinetic analysis to be conducted by following
product formation. Adiabatic heating or cooling effects commonly associated with HHP
62
systems upon pressurization and depressurization were not significant factors as the
temperature controlled jacket limited temperature fluctuations to less than 2 °C.
Because the high pressure reactor was closed pressure increased simultaneously with
temperature. When temperature reached 68.7 ºC (hexane boiling point at ambient
pressure) pressure had already reached 5 MPa. In other words, during the heating of
the reaction cell, because of the simultaneous increase in pressure, hexane never
reached the boiling point. Within the context of this study, pressures below 10 MPa,
reached under these conditions, are referred as “low pressures”. Pressure and
temperature effects on the reaction, in the absence of enzyme, were ruled out when no
significant reaction progress was observed at pressures up to 700 MPa and 80 ˚C for 4
hr (data not shown) which was similar to previous studies [224] whereby isoamyl
acetate production was negligible in absence of a catalyst. Native lipase activity was
determined by assaying lipase that has not been exposed to temperatures above
recommended storage conditions (5 °C). Percent relative activity was determined by
comparing the initial rate of the observed reaction to that of the native enzyme (control).
Samples were treated and assayed in a randomized block design, blocked by
temperature and incubation time while pressure varied. Significant differences in
treatments were determined using analysis of variance (ANOVA) and Tukey’s pair-wise
comparison at α = 0.05 for enzyme treatments and controls. Statistical analysis was
done using SAS software (Cary, NC USA).
Comparison of application of HHP and heat methods
Three sequences of application of pressure and heat were utilized to compare
changes in enzyme activity derived from non-inactivating conformational enzyme
changes. Such changes were assessed thought the determination of rate constants and
63
activation energies. Application sequences were pressurization first, simultaneous
heating and pressurization, and heating first as shown in Fig. 2-2. In all cases,
incubation time began when the desired pressure was achieved (± 10 MPa) and at least
90% of the difference between cold temperature and incubation temperature were
reached. Controls (100% activity) correspond to the activity after reaching set-point
temperature and pressure then depressurization and cooling with no incubation period.
Apparent initial rate was determined by mixing 2.5 ± 0.1 mg immobilized lipase and 2
mL of isoamyl alcohol and acetic acid 0.06 M in hexane in the reaction vial and
immediately inserted into the reactor. Pressure (0.1 to 400 MPa) and temperature (36,
42, 48.9, 56.2, 63.5, 71.8, 80 ± 0.1 °C) were adjusted according to method of
application as previously discussed and shown in Fig. 2 and compared to assays at low
pressure . The reaction vial was held at 5 °C ± 0.1 °C prior to and after incubation
conditions. During incubation the reaction mixture was stirred with the magnetic stir bar.
Upon completion of incubation cycle the reaction vial was removed and a 1-μL aliquot
was taken for GC-FID analysis at time intervals of 0, 2.5, 5, 7.5, and 10 min. Rate was
determined from the slope of the linear regression (R2 > 0.95) of the time course
production of isoamyl acetate by fitting product concentration vs. time. Reaction rate
was expressed as concentration (mmol L-1) isoamyl acetate generated per second.
Arrhenius plots were used to determine the initial reaction rate dependence on
temperature between 36 and 80 °C and calculate Ea. Statistical comparisons of
treatment methods were conducted using SAS statistical software (Cary, NC USA)
utilizing GLM regression analysis.
64
Activation volume
Pressure effects on initial rate were examined at 0.1 to 600 MPa at 40 or 80 °C.
Initial rate was determined by mixing 2.5 ± 0.1 mg immobilized lipase and 2 mL of
isoamyl alcohol and acetic acid 0.06 M in hexane in the reaction vial and immediately
inserted into the reactor. Rate was determined from the slope of the linear regression
(R2 > 0.95) of the time course production of isoamyl acetate by fitting product
concentration vs. time. Reaction rate was expressed as concentration (mmol L-1)
isoamyl acetate generated per second.Pressure and temperature treatments were
applied using the “pressure-first” method described in section 2.2.2. The effects of
pressure on enzyme activity are described by an overall activation volume (ΔV≠)
determined from Eyring’s equation (shown in Chapter 1, equation 1-1).
where k is the equilibrium constant, p the pressure, T the absolute temperature, R
the gas constant and ΔV≠ the activation volume [225].
Electron micrographs of immobilization beads
Scanning electron microscopy (SEM) was utilized to examine the solvent,
temperature, and pressure effects on the immobilization support (macro porous acrylic
resin) shape and conformation as well as the surface texture. Samples were dried at 40
°C for 30 min before a 90-s application of gold palladium coating. Incubation treatments
included a control (no treatment), exposure to hexane for 4 h, exposure to hexane and
80 °C for 4 h, and exposure to hexane at 80 °C and 400 MPa for 4 h, and after assaying
with and without hexane, heat, and pressure treatment.
65
Results and Discussion
Effect of HHP on Lipase Stability
Immobilized lipase was incubated at 80 °C and from 10 to 700 MPa for 4 h.
Results are shown in Fig. 2-3. Residual activity at ambient pressure after the 4-h
treatment was 40%. Relative residual activity increased with pressure until reaching a
maximum at around 400 MPa where residual activity was around 99%. Pairwise
comparison of enzyme treatment and controls using Tukey’s test (α = 0.05) allowed
determination of significant differences between pressure treatments. Residual activity
was significantly higher above 300 MPa compared to at 10 MPa. Residual activity at
400, 600, and 700 MPa was significantly higher than at 100 MPa. Compared to
incubations at ambient pressure at 80 °C for 4 h, at 400 MPa thermal inactivation of
lipase was reduced by up to 152%. The confidence intervals are larger than desired due
to experimental error associated with difficulties in measuring small quantities of
immobilized enzyme (10 mg) beads with different surface area on which lipase is bound
[226]. The largest surface area of the immobilization bead was 4-fold that of the
smallest. Therefore, changes in surface area greatly affect the total number of enzyme
units per weight of beads. Residual activity near or slightly above 100% at 400 MPa
may be due to pressure and heat induced conformational changes in the lipase allowing
greater activity post-incubation but most probably are simply the result of experimental
error described above. In order to clarify this issue in situ conformational studies are
needed to observe structural changes which may be occurring during come-up time,
incubation time, and come-down time. Similar studies have been conducted at elevated
pressure using fluorescence spectroscopy [169], derivative spectroscopy [227], x-ray
scattering [228], and quantitative Raman spectroscopy [229]. To conduct these studies
66
with CALB, the enzyme must be solubilized in hexane using a synthetic detergent
according to Tsuzuki et al.[230], and require different specialized HHP optical cells
depending on the method used.
Pressure induced stabilization was also shown for a similar from Rhizomucor
miehei lipase in soluble form in aqueous solution as well as invertase from
Saccharomyces cerevisiae [106]. At denaturing temperatures (50, 55, and 60 °C)
application of pressure protected the lipase at a range of 50 to 350 MPa by increasing
residual activity from about 82 to 95% at 50 °C, about 32 to 70% at 55 °C, and from 0
to about 35% at 60 °C [106]. The protective effect of pressure increased with pressure
up to 150-250 MPa with more pronounced stabilization effects as temperature
increased from 40 to 60 °C. In the same study, it was observed that invertase half-life
increased until pressure reached 200 MPa, meaning that the enzyme was protected by
pressure in the range of 50-200 MPa and beyond 200 MPa residual activity decreased
[106]. This phenomenon is also similar to that of pectin methyl esterase (PME) which
showed an increase in optimal temperature from 45 to 55 ºC as the pressure increased
from 0.1 MPa to 300-500 MPa) [99].
These stability studies indicate that pressure significantly stabilizes the
immobilized lipase up to 400 MPa. Recently, the activity of lipases from porcine
pancreas, Candida antarctica, Candida cylindracea (immobilized), Penicilium roqueforti,
Aspergillus niger, Rhizopus arhizus, Mucor miehei, and Pseudomonas cepacia was
studied after hydrolysis under SC-CO2 at 40 °C and 15 MPa [171]. All lipases tested had
increased relative activity with the greatest increase from Rhizopus arhizus lipase which
was increased by more than 50 times while Candida antarctica lipase activity increased
67
from 0.32 to 5.97 U g-1 after treatment in SC-CO2 and up to 21.00 U g-1 during exposure
to SC-CO2. However, these results contrast to previous studies of lipase in supercritical
carbon dioxide (SC-CO2) and compressed n-butane which showed increased activity as
pressure increased up to 35 MPa [50, 104, 109] with a precipitous drop beyond that.
Although the mechanism of HHP induced stabilization has yet to be fully
elucidated, it appears that pressure effects on intramolecular interactions, hydration of
charged groups, disruption of bound water, and stabilization of hydrogen bonds may all
play some role. According to Mozhaev et al. [125], the antagonistic effects of pressure
and temperature rests upon counteracting effects on the ability of functional groups to
interact with water. Pressure enhances the hydration of charged groups, whereas the
hydration of charged groups is loosened at high temperature [30]. Furthermore,
opposing effects of pressure and temperature with respect to hydrophobic interactions
and hydrogen bonds offer a possible explanation for pressure stabilization of enzymes
against thermal inactivation [91]. Endothermic hydrophobic interactions are known to be
enhanced at elevated temperatures, being maximal at about 60-70 °C and thereafter
decreasing because of a gradual breakdown of the water structure [231]. Hydrogen
bridges are generally known to be stabilized by pressure and destabilized by heat [231,
232]. These cumulative antagonistic effects of pressure and heat may offer explanation
of pressure induced resistance to thermal inactivation.
Pressure induced stabilization is contrary to pressure effects of a similar lipase
from R. miehei in aqueous solution. According to Noel et al [169] pressure treatment
under 450-500 MPa at 25 °C had equivalent inactivation rates as thermal treatment at
50-55 °C. These apparent conflicting results may be contributed to various different
68
incubation conditions, mainly enzyme immobilization and solvent polarity as well as
inherent differences in the lipases tertiary and secondary structures. However, in the
same study Noel et al. [169] concluded that lipase has a high stability under pressure as
represented by a slight change in enzyme volume (0.2%) in comparison to initial volume
of the native protein. Furthermore, it was concluded that the application of high pressure
combined or as an alternative to high temperature is of immediate relevance to
modulate enzymatic activity [169].
Comparison of Pressurization and Heating Methods on Activation Energy
Initial rate of isoamyl acetate production using each method at 400 MPa and 36 to
80 °C was compared to assays at low pressure. Apparent initial rate results are shown
in Table 2-1 and summarized with percent change as compared to rates at low
pressure. In all sequences activity at 71.8 or 80 °C and 400 MPa was greater than at
low pressure by 19.8 to 96.1% depending on the method and temperature. Activation
energy (Ea) was determined for each of three methods. At temperatures above 63.5 ºC
Arrhenius plots deviated from linearity, indicating that unlike in the stability study in
section 3.1, in the presence of substrate, lipase inactivation may be occurring. In the
time frame of these experiments the rates of reaction still increased with temperature. In
contrast, at ambient pressure, activity decreased with increasing temperature above
63.5 ºC. Therefore, Ea was determined in the range of 36 to 63.5 °C. Ea at low pressure
and was 42.7 ± 3.60 kJ mol-1. The pressure-first, simultaneous, and heat-first methods
had Ea of 42.36 ± 6.9, 47.8 ± 8.16, and 35.7 ± 3.5 kJ mol-1 respectively. No significant
differences were found in Ea at any pressure tested irrespectively of the pressurization
and heating sequence. This contrasts with the findings of Weemaes et al. [91] who
found that Ea varied with hydrostatic pressure for polyphenoloxidase, whereby it was
69
found that activation energy decreased with increasing pressure. The heat-first method
consistently resulted in slightly higher rates than all other methods tested at all
temperatures as shown in Table 2-1. This is most likely because temperature was
consistently higher at the beginning of the incubation time using the heat-first method,
while incubation time started when temperature reached 90% of the set point for the
other two methods while for the heat-first method, pressurization time allowed heating to
about 95% of the set point. CALB in n-hexane using acetic anhydride (a more effective
acyl donor) resulted in lower Ea (11.3 kJ mol-1) [38] for synthesis of isoamyl acetate. Ea
was slightly higher to that reported in a solvent free system (28.7 kJ mol -1) [47] and in
biphasic-ionic liquid (27.3 kJ mol -1) [52]. These results are similar to other ester
synthesis reactions catalyzed by CALB; including butyl butyrate (32 kJ mol-1) in SC-CO2
[157] and tetrahydrofurfuryl butyrate (47 kJ mol -1) [233], oleyl oleate (37 kJ mol-1)[234],
butyl laurate (45 kJ kJ mol-1)[234], butyl oleate (37 kJ kJ mol-1)[234], and oleyl
butanoate in hexane (39 kJ mol-1) [234].
Several enzymes have shown enhanced activity while or after exposure to HHP;
including polyphenoloxidase [88, 96], pectin methylesterase [97, 99], α-chymotrpisn
[125], dehydrogenase [83, 84], protease [20], α-amylase [114], peroxidase [88],
thermolysis [129], and pepsin [129] among others. Several reasons for pressure-
induced changes in the rate of enzyme catalyzed reactions have been offered and are
classified into three groups: (1) changes in the structure of an enzyme; (2) changes in
the reaction mechanisms; for example, a change in the rate-limiting step; and (3)
changes in the substrate or solvent thus affecting enzyme structure or the rate limiting
step.
70
Enzymatic conformation is affected by both pressure and temperature, thus
affecting activity. CALB is a monomeric enzyme and there is evidence that activities of
monomeric enzymes are stimulated while the activities of multimeric enzymes are
inhibited by application of high hydrostatic pressure [56]. However, at least fifteen
dimeric and tetrameric enzymes that are activated by pressure have been reported [32].
Noel et al. [169] compared conformational changes at elevated pressure (300 - 500
MPa) to those at elevated temperatures (40 - 60 °C) by measuring emission spectrum
at 290 and 350 nm for R. miehei lipase. Conformational changes induced by pressure
were attributed to aggregation (increased fluorescence at 290) and were different from
those induced by temperature, attributed to unfolding (increased fluorescence at 350).
In both cases decreased activity was reported.
Activation Volume Determination
Effect of pressure on the initial rate (Vmax) of lipase catalyzed isoamyl acetate
formation at 40 and 80 °C is shown in Fig. 2-4. Activity was higher at 80 ºC than at 40
ºC at all pressures. At 80 ºC Vmax increased with pressure in the range of 0.1 to 300
MPa followed by a decrease in the range of 350 to 600 MPa. At 40 ºC Vmax increased
with pressure in the range of 0.1 to 100 MPa followed by a decrease in the range of 200
to 600 MPa. Activities at 100 to 400 MPa at 40 ºC and at 100 to 450 MPa were higher
than at low pressure. Maximum rate of reaction was 2.09 x 10-3 at 300 MPa and 80 ºC.
This pressure was below that of maximum stability (400 MPa) discussed previously.
Reversible enzyme denaturation may account for this decrease because, unlike in the
stability studies where pressurization was done in the absence of substrate and activity
assays were carried out ex-situ, the progress of this reaction occurred under pressure in
71
the presence of substrate. This provides insight into the effects of the presence or
absence of substrate on lipase stabilization.
The relationship between pressure and the logarithm of Vmax was linear between
300 and 500 MPa at 40 and 80 °C. Therefore, the effect of pressure on the reaction rate
was described using the Eyring equation to determine ΔV≠ as shown in Fig. 5. ΔV≠
slightly increased with temperature from 14.3 ± 1.7 to 15.2 ± 2.2 cm3 mol-1 at 40 or 80
°C, between 300 and 500 MPa. These results were not significantly different.
Interestingly, apparent ΔV≠ was negative from 0.1-200 MPa at 80 °C and from 0.1- 100
MPa at 40 °C. At pressure below 400 MPa inactivation occurred at 80 °C as previously
shown in Fig. 2-3. Therefore, at 80 °C below 400 MPa the apparent negative ΔV≠ may
be attributed to partial enzyme inactivation. Pressure induced stabilization offers a
possible explanation for the increased activity at 80 °C, but not at 40 °C whereby the
lipase is considered stable [38]. Therefore, both enzyme stabilization and pressure
activation might be occurring simultaneously. Recently carrot pectin methyl-esterase
(PME) showed very similar effects while at range of temperature (30–60 °C) and
pressures ( 0.1–600 MPa) [101]. The PME showed a negative ΔV≠ below 400 MPa at
temperature greater than 60 °C and a positive ΔV≠ above 400 MPa at all temperatures
tested [101].
To the best of our knowledge there are no other reports on the effects of HHP on
CALB in organic media. However, the effect of high pressure in SC-CO2 on the isoamyl
acetate synthesis from isoamyl alcohol using CALB was reported by Romero et al.
[161]. Pressure had no significant influence on esterification of isoamyl acetate between
8 and 30 MPa at 40 °C. This may be attributed to the relatively low and narrow pressure
72
range used by that group. In another study, Pseudomonas cepacia lipase (PCL)
catalyzed transesterification of 1-phenylethanol with vinyl acetate in SC-CO2 showed an
increase in catalytic efficiency up to 15 MPa. However, ΔV≠ did vary with pressure range
used, reaching a maximum negative value of -1340 cm3 mol-1 at 7.4 MPa [55]. High
negative ΔV≠ would be expected in SC-CO2 at this narrow pressure range (0.1–15 MPa)
due to changes in solvent phase and density as well as solubility and partitioning of
substrates but not as direct effect on enzyme activity.
Lipase activity may be higher between 100 and about 350 MPa compared to at
low pressure due to a shift in the tertiary structure surrounding the active site allowing
greater substrate interaction. Crystallographic and molecular-modeling studies of CALB
determined that lipase belongs to the α/β hydrolase fold family with a catalytic triad
consisting of Ser, His, and Asp/Glu [172]. Early X-ray diffraction data suggests that a
lipase’s helical part of the α-helix near the active site forms a “lid” that rotates almost
90°, from lying flat on the surface to extending nearly perpendicular to it on
rearrangement to the open conformation [173]. However, recent studies conducted in
aqueous media have concluded that in contrast to most lipases, CALB may not have a
“lid” covering the entrance to the active site and shows no interfacial activation [68] as
compared to Candida antarctica lipase A (CALA) which does possess the characteristic
“lid” structure and shows interfacial activation [174]. Furthermore, flexibility of CALB is
reduced in organic solvents, and is limited to: (1) a short α-helix which form the entrance
to the active site, (2) three surface loops, (3) the medium binding pocket for secondary
alcohols, (4) the acyl binding pocket, and (5) the large binding pocket for secondary
alcohols [68]. Flexibility limited to these five elements vital to catalysis may offer
73
possible explanation for relatively high pressure stability, while still allowing modification
of activity. Although flexibility is limited in organic solvents, to the best of our knowledge
the effects of pressure on the flexibility of these five elements or other modifications of
the active site have not been explored in organic solvents at HHP.
Pressure effects on proteins and enzymatic reactions have been discussed and
reviewed in depth over the past 20 years [16, 18, 19, 28-31, 235]. It is understood that
pressure effects on catalysis reactions are related to Le Chatelier’s principle: elevated
pressures favor changes that reduce a systems overall volume. Thus, by comparing the
total volumes of the reactants versus products, of the ground state versus activated
state, or of the dissociated versus bound complex, the effect of pressure on reaction
equilibria or rates can be estimated [28]. HHP increases substrate concentration as a
result of a decrease in volume thus increasing reaction rate. Concurrently HHP
increases solvent viscosity hindering reaction rate. In this study viscosity effects may be
negligible due to constant vigorous agitation during incubation and activity assays. In
contrast to simple chemical reactions, it is difficult to give a precise interpretation of
calculated ΔV≠ for enzymatic synthesis reactions because pressure affects several
factors including: enzyme conformation, enzyme solvation (interaction with surrounding
medium, other proteins, water, ions, etc.), immobilization matrix, etc. Furthermore,
neither positive nor negative activation volumes seem to be predominant in enzyme
reactions. Typically, however, ΔV≠ ranges from -70 cm3 mol-1 to 60 cm3 mol-1 with most
being less than 30 cm3 mol-1 [28] which is in agreement with the findings of this study.
The pressure dependence of the solubility parameter and molar volume (among
others) of hexane has been recently described at pressures up to 300 MPa at 30 °C.
74
Pressure monotonically increased the solubility parameter (~20%) and decreased the
molar volume (16%) [66]. It was determined that use of more non-polar solvents on the
synthesis of isoamyl acetate results in better esterification as they preserve the catalytic
activity without disturbing the micro aqueous layer of the enzyme [67]. Pressure
increases hexane’s solubility parameter thus may be antagonistic to the esterification of
isoamyl acetate because esterification is favored in less polar solvents. However, the
flexibility of CALB is increased with increasing polarity of the organic solvent [68].
Therefore, pressure may increase flexibility of CALB.
Lipase activity in organic solvents was correlated with the solvent polarity [40].
However it has also been reported that lipase activity might be affected by the solvent
without correlation to the polarity [79, 80]. Lipases that are active in organic solvents
retain their native structure upon transfer from water to organic solvents [70, 71].
However, it is essential to have small amounts of water to maintain stability and
flexibility of lipases in organic solvent. Thus, enzyme-bound water is essential for
catalysis and serves as a lubricant for the enzyme. In contrast, fully dry enzymes are
inactive and enzymes in organic solvents with high amounts of water show denaturation
[64, 73]. Since pressure has been shown to enhance the hydration of charged groups
one can hypothesize that pressure helps to maintain bound water, therefore enhancing
activity. These pressure dependent changes of the reaction medium and their effects on
lipase stability and activity remain unclear and need further exploration.
Electron Microscope Examination of Immobilization Beads
In an effort to isolate HHP effects on lipase versus the effects on the
immobilization support, scanning electron microscope (SEM) images were taken of the
immobilized lipase at various stages throughout the treatments. It was hypothesized
75
that increased activity may be generated from deformations, cracking, or splitting of the
immobilization support. This was not found to be the case as Fig. 6 shows the SEM of
immobilization supports (macro porous acrylic resin beads) before (Fig. 6A) and after
(Fig. 6B) exposure to hexane at 80 °C and 700 MPa for 4 h magnified to examine shape
of resin bead and bead surface. The immobilization supports were also examined after
assay without incubation (Fig. 6C) and after assay at 80 °C and 700 MPa for 15 min
(Fig. 6D). These results indicate that no visible change has occurred in either the overall
shape or in the surface texture of the immobilization bead as compared to the control
and to previous studies [226]. Surface differences do appear in Fig. 6A and 6B due to
orientation of the bead during imaging. Also, differences can be seen when comparing
Fig. 6A, B and Fig. 6C, D due to residue on the surface. These visible residues may be
attributed to assay effects on the immobilization support. There was a large variation in
size of immobilized beads. The largest bead was approximately 500 µm while the
smallest was approximately 125 µm. This variation in diameter corresponds to a 4 fold
variation in surface are. Lastly, presence of some cracked or broken beads were seen
equally in both controls and treatments. The lack of a significant change in bead shape
or surface contour adds further evidence towards confirming that pressure, temperature,
and solvent effects are acting directly on the enzyme and not physically distorting the
immobilization support which could result in apparent improved activity. However, it
remains a possibility that the immobilization support is distorted while under pressure
and returns to original conformation upon depressurization. Changes in the structural
integrity of immobilization supports may be monitored in situ at elevated pressure by
76
using high pressure optical cells with diamond or sapphire windows [228, 229] which
allow continuous monitoring.
Conclusions
Previous studies [38, 42, 221] indicate that the optimal conditions for isoamyl
acetate formation using lipase in hexane at atmospheric pressure was 43.2 °C. This
study indicates the optimal thermal conditions of this reaction may be dramatically
increased by the implementation of HHP. The results of this study suggest that the
stabilization and catalytic improvement effects of HHP have potential for various
applications to lipase-catalyzed production of isoamyl acetate.
While enzymatic enhancement clearly occurs up to 400 MPa, the effects beyond
this pressure are not fully understood. Many areas remain to be investigated including
the mechanism of HHP induced stabilization and increased or decreased activity, HHP
effect on other immobilized and free lipases, effects of HHP during extended incubation
times (> 4 h), and a complete optimization of HHP utilization for isoamyl acetate
synthesis. While the relationship between elevated pressure and temperature effects on
lipase remain to be completely resolved, it is clear that HHP is a useful reaction
parameter for improving lipase catalysis.
This study illustrates the complexity of enzyme kinetics at a range of pressures. As
opposed to simple chemical catalysis, the apparent activation volume may appear
positive or negative depending on the pressure effects on enzyme conformation,
temperature-pressure antagonistic effects, solvation effects, as well as pressure effects
on the chemical equilibrium.
77
Acknowledgments
This project was supported by a Research Innovation Grant from the University
of Florida Institute of Food and Agricultural Sciences. The authors are grateful for the
assistance of Mrs. Diane Achor of the Citrus Research and Education Center, Electron
Microscopy Laboratory, and to James Colee of the Institute of Food and Agricultural
Sciences statistical group.
Time ( s )
A
B
C
[----------- Incubation ----------]
Figure 2-2. Temperature (circle) and pressure (triangle) profiles for (A) “Pressure-First”, (B) “Simultaneous”, and (C) “Heat-First” method for a 10 minute incubation at 80 °C and 400 MPa.
78
Pump Controller
Wat
er B
ath
(Coo
l)
Wat
er B
ath
(Hea
t)
Monitoring Software
Reac
tor
Magnetic Stirrer
Reactor Cap
Hydraulic Fluid Line
High Pressure Pump
Reaction Vial
Figure 2-1. Schematic representation of the high hydrostatic pressure system.
Figure 2-3. Effect of high pressure on enzyme stability after incubation for 4 h at 80 °C. Assayed with 10 ± 0.5 mg lipase, 0.06 M substrate. Error bars represent a 95% confidence interval using analysis of variance.
79
0.0E+00
1.0E-02
2.0E-02
3.0E-02
4.0E-02
0 100 200 300 400 500 600
Vm
ax
(m
mo
l ∙
L-1
∙ s
-1)
Pressure (MPa)
Figure 2-4. Effect of pressure on Vmax at (●) 40 °C and (■) 80 °C for lipase-catalyzed production of isoamyl acetate (Novozyme 435 in n-hexane ) using the “pressure-first method”. Error bars represent standard error of the slope of apparent the initial rate calculated from linear regression using a 95% confidence intervals.
-6
-5.5
-5
-4.5
-4
-3.5
-3
-2.5
0 100 200 300 400 500
ln V
ma
x
Pressure (MPa)
Figure 2-5. Determination of activation volume using the Eyring equation at (●) 40 and (■) 80 °C for lipase catalyzed production of isoamyl acetate using the “pressure-first method”.
80
Figure 2-6. Scanning electron micrographs of the surface of Lipozyme® (Novozyme L4777) immobilized on acrylic resin (A) before and (B) after exposure to hexane solvent at 80 °C and 700 MPa for 4 h and after assay (C) without incubation and (D) with incubation at 80 °C and 700 MPa for 4 h treatment. Inserts illustrate the retention of bead integrity after different treatments.
81
Table 2-1. Initial rate and percent change using various “pressure first”, “heat first”, and “simultaneous” methods of applying heat and pressure as compared to assays at low pressure.
Low Pressure Pressure First
(400 MPa) Heat First (400 MPa)
Simultaneous (400 MPa)
Temp (˚C)
Initial Rate (mmol L
-1sec
-1)
Pressure (MPa)
Initial Rate (mmol L
-1sec
-1) % Change
Initial Rate (mmol L
-1sec
-1) % Change
Initial Rate (mmol L
-1sec
-1) % Change
36.0 5.31 x10-3
0.1 4.49 x10-3
-15.4 8.97 x10-2
68.8 4.26 x10-4
-19.7 42.0 7.45 x10
-3 1 4.50 x10
-3 -39.6 1.05 x10
-2 40.7 3.73 x10
-4 -49.9
48.9 1.00 x10-2
2 9.32 x10-3
-6.8 1.33 x10-2
32.7 7.68 x10-4
-23.2 56.2 1.69 x10
-2 6 1.02 x10
-2 -40.4 2.15 x10
-2 26.5 1.16 x10
-4 -31.9
63.5 1.94 x10-2
7 1.62 x10-2
-16.3 2.59 x10-2
33.9 1.63 x10-4
-16.4 71.8 1.60 x10
-2 8 1.91 x10
-2 19.8 2.90 x10
-2 81.3 1.95 x10
-3 21.9
80.0 1.57 x10-2
10 2.49 x10-2
43.2 3.08 x10-2
96.2 2.38 x10-3
51.6
* Bold font indicates a pressure-induced positive increase in activity. * Increasing pressure for “Low Pressure” treatment is due to heating of the sealed HHP system with the pump off.
82
CHAPTER 3 ACTIVATION VOLUME AND APPARENT MICHAELIS MENTEN PARAMETERS OF
LIPASE AT HIGH HYDROSTATIC PRESSURE IN HEXANE WITH EXCESS ALCOHOL
Introduction
Kinetic studies of lipase-catalyzed reactions in hexane have proposed a Ping-
Pong Bi-Bi mechanism shown in Equation 3-1 [221], and operating conditions such as
acyl donor, type of lipase, and temperature have been optimized [38]. Also, evidence of
HP enzyme enhancement and possible mechanisms of stabilization and activation have
been reviewed and discussed in chapter 1. Although chapter 2 has documented the
activation energies (Ea) and activation volume (ΔV‡) of inactivation, no work has
focused on investigating the ΔV‡ of activation or other kinetic parameters of lipase
catalyzed synthesis of isoamyl acetate in an organic solvent at HHP. Kinetic parameters
are necessary for further optimization of temperature and pressure conditions while
utilizing lipase catalyzed synthesis at elevated pressure. Furthermore, by characterizing
the ΔV‡ of activation the mechanism of pressure induced activation can be explored
further. The objective of this research was to determine the effects of pressure on
increasing the overall reaction rate and on enzyme-substrate (acetic acid) binding in
excess alcohol. To achieve this objective the apparent Michaelis Menten parameters
and the ΔV‡ of activation for the synthesis of isoamyl acetate in hexane catalyzed by
immobilized lipase at HHP was determined.
Materials and Methods
Materials
Lipase (Novozyme 435® E.C. 3.1.1.3) from Candida antarctica lipase B (CALB)
expressed in Aspergillus oryzae immobilized on a macro porous acrylic resin (13,100
83
PLU/g) was obtained from Sigma Aldrich (St. Louis, MO USA). Isoamyl alcohol, glacial
acetic acid, and HPLC grade hexane were obtained from Fisher Scientific (Pittsburg, PA
USA). All solvents and substrates were held at -10 °C or on ice while preparing for
assay. Reaction vials were made using 3-mL syringes with Luer-Lock™ tips (BD Franklin
Lakes, NJ USA) which allowed substrate insertion with an opposing plunger while
preventing solvent, substrate, or enzyme leaching during pressurization.
The HHP system consisted of a high pressure reactor (model U111), a high
pressure micropump (model MP5), and a pump controller (MP5 micropump control unit)
all from Unipress Equipment (Warsaw, Poland). The reactor was temperature-controlled
with a water jacket alternatively fed by two water baths (Isotemp 3016D); one cooling (5
or 10 °C) and another heating (25 to 80 °C ± 0.1 °C) from Fisher Scientific and
controlled by an array of pinch valves. Computer programs written in LabVIEW and a
data acquisition board (DAQ Card 6062E) from National Instruments (Austin, TX USA)
were used to collect temperature and pressure data and to control the heating/cooling
valve array. A depiction of the HHP system has been previously described in chapter 2
and is pictured in Appendix 1. Stirring inside the reaction vial was initiated by a
magnetic stir-bar inside the reaction vessel and controlled by external spinning
neodymium magnets on an AC motor type NS1-12 (Bodine Electric Company, Chicago,
IL USA). Reaction progress was monitored using GC-FID 5890 (HP, Palo Alto, CA
USA) with a ZB-5 column (30 m length × .53 mm ID × 1.5 μm thickness) at a gradient
temperature from 50 °C to 90 °C at 5 °C min-1. Injector temperature was held at 200 °C
and FID detector at 250 °C.
84
Methods
Determination of lipase catalyzed isoamyl acetate production rate
Enzyme was weighed (2.5 mg or ~128 Propyl Laureate Units) into the reaction vial
with a miniature stir bar. The reaction mixture (solvent and substrates, described in
sections 2.2.2 and 2.2.3) was added to the reaction vial to initiate the reaction. The
reaction vial plunger was moved into position to eliminate air bubbles then sealed with a
Leur-lock™ plug. The reaction vial was then placed in the high pressure reaction
chamber being held at 5 °C. Polydimethylsiloxane silicone liquid (Accumetric, Inc.,
Elizabethtown, KY USA) was added as hydraulic fluid to fill the reactor. The reactor was
sealed and pressurized. After pressure reached the set-point, temperature was adjusted
to the set-point. Upon completion of incubation, the temperature was returned to 5 °C,
and the reactor was depressurized and opened. The reaction vial was withdrawn.
Lipase activity was determined by monitoring the reaction progress of the esterification
of isoamyl alcohol and acetic acid to form isoamyl acetate as previously described [38,
168, 221] and shown as
Pressure and temperature treatments were applied using the “pressure-first”
method shown in Fig 3-1. and using the high pressure system previously described
[168].
Determination of activation volume
Pressure effects on initial rate were examined between low pressure (between 1
and 10 MPa) and 600 MPa at 40 or 80 °C. Initial rate was determined by mixing 2.5 ±
0.1 mg immobilized lipase and 2 mL of isoamyl alcohol and acetic acid 0.06 M in
hexane in the reaction vial and immediately inserted into the reactor. Rate was
determined from the slope of the linear regression (R2 > 0.95) of the time course
85
production of isoamyl acetate by fitting product concentration vs. time. The effects of
pressure on enzyme activity were described by an overall activation volume (ΔV≠)
determined from Eyring’s equation (shown in Chapter 1, equation 1-1).
Determination of apparent Michaelis-Menten parameters
Apparent KM and Vmax were determined at low pressures (between 1 and 10
MPa) and at 200 MPa at 40 ˚C or 80 ˚C. Initial rate was determined by mixing 10 ± 0.1
mg immobilized lipase and isoamyl alcohol and acetic acid in hexane in the reaction vial
and immediately inserting it into the reactor. Isoamyl alcohol concentration remained
constant (5.0 X 10-1 M, in excess) while the acetic acid concentration varied from 5.0 X
10-3 to 2.5 X 10-1 M. Rate was determined from the slope using linear regression (R2 >
0.95) of the time course production of isoamyl acetate by fitting product concentration
vs. time. Apparent KM and Vmax were determining using Lineweaver-Burk approximation.
Although conventional synthesis of isoamyl acetate is conducted at acid-alcohol
ratios of 1:1 [221], in this study excess of non-inhibitory isoamyl alcohol is utilized to
determine the apparent KM and Vmax by reducing the Ping-Pong Bi-Bi mechanism
reaction shown in Figure 3-2 to an apparent one substrate, one product Michaelis
Menten kinetics.
Results and Discussion
Activation Volume
The effect of pressure on the initial rate (Vmax) of lipase catalyzed isoamyl acetate
formation at 40 and 80 °C is shown in Fig. 3-3. Activity was higher at 80 ºC than at 40
ºC at all pressures. Activity was also higher at elevated pressures than at low pressure
up to 400 MPa at 80 ˚C and up to 350 MPa at 40 ˚C. At 80 ºC initial rate increased from
10 to 250 MPa, remained relatively constant between 250 and 350 MPa, then
86
decreased from 350 to 600 MPa. At 40 ºC Vmax increased from 1 to 100 MPa, remained
relatively constant between 100 to 200 MPa, and then decreased from 200 to 600 MPa.
The relationship between pressure and the logarithm of Vmax was determined in
the linear ranges between 1 to 100 MPa at 40 ˚C and between 10 to 150 MPa at 80 ˚C
as shown in Fig. 3-4. The ΔV‡ values are summarized in table 3-1. For both
temperatures increasing pressure initially increased reaction rates to a point where
higher pressures decreased reaction rates as indicated by negative and positive ΔV‡
values respectively. Temperature did affect ΔV‡ at low pressure but did not at high
pressure (as shown in Chapter 2); indicating that pressure induced activation is affected
by temperature while inactivation is not. This may be explained by pressure weakening
or strengthening intra or intermolecular bonds or modifying vital structural motifs. These
modifications can lead to either greater exposure (i.e. activation at low pressure), or
concealment (i.e. inhibition at higher pressure) of the active site. For example, as
discussed in chapter 1, hydrogen bonds are weakened by high temperature and
strengthened by high pressure. Therefore, at lower temperature, this strengthening of
hydrogen bonds as pressure increases (from 0.1 to 100 MPa) may have a pronounced
effect on the active site. This effect would then be diminished by the disruption effects of
elevated temperature (at 80 ˚C) and result in a less negative ΔV‡. Likewise, the effect of
increasing pressure above 300 MPa may have overriding effects on structurally vital
bonds that result in the same positive ΔV‡ regardless of temperature.
The negative ΔV‡ found in this study is similar to another lipase from
Pseudomonas cepacia (PCL). PCL catalyzed transesterification of 1-phenylethanol with
87
vinyl acetate in SC-CO2 showed an increase in catalytic efficiency up to 15 MPa. Also,
ΔV≠ did vary with pressure range used, reaching a maximum negative value of -1340
cm3 mol-1 at 7.4 MPa [55]. High negative ΔV≠ would be expected in SC-CO2 at this
narrow pressure range (0.1–15 MPa) due to changes in solvent phase and density as
well as solubility and partitioning of substrates but not as direct effect on enzyme
activity.
Because the activation energy (Ea) is constant regardless of the pressure (as
shown in Chapter 2), to properly model the effects of pressure and temperature on
reaction rate simultaneously, a function of ΔV≠ versus temperature is required. Such
functions have been proposed and generated for thermal and pressure inactivation of
PPO by Weemaes and others [91] and for actinidin by Katsaros and others [236]. A
polynomial function describing the effects of pressure on rate at different temperatures
was substituted into the Arrhenius equation. According to Weemaes, the proposed
model accurately described the empirical data within the range tested. However, in
contrast to this study, both Weemaes and Katsaros found that Ea of inactivation was
affected by changes in pressure. These differences in pressure-temperature effects
may be attributed to different enzymes and differences in the temperature-pressure
combinations. Therefore, as a general rule it must be considered that over a broad
enough temperature or pressure range, changing temperatures will always affect ΔV≠
and changing pressures will always affect Ea.
Michaelis-Menten Parameters
Effect of pressure and temperature on the Michaelis-Menten parameters KM and
Vmax at 40 or 80 ˚C and low pressure or 200 MPa is shown in Table 3-2 and in Fig 3-5.
88
Pressure significantly increased Vmax at both temperatures by approximately 10-fold.
Pressure induced increases in Vmax is in agreement with previous results (chapter 2)
that demonstrated the effect of pressure induced rate increases on lipase catalyzed
isoamyl acetate synthesis in hexane. Vmax was greater at 40 ˚C and 200 MPa than at
80 ˚C and 0.1 MPa. The lipase may be undergoing thermal induced inactivation at 80 ˚C
and 0.1 MPa since according to the results in chapter 2, at pressure below 400 MPa,
lipase inactivation occurs at 80 °C.
Increasing pressure increased KM at 40 ˚C by 14-fold which indicates a decrease
in affinity between the CALB and acetic acid. Although this decrease in affinity can slow
the overall reaction velocity, these effects are lessened or null when pressure
simultaneously increases the product release (Vmax, which is typically the slow/limiting
step). At 80 ˚C KM was not affected by pressure which indicates that the formation of the
enzyme-acid complex is being hindered at 40 ˚C but not at 80 ˚C. The conformational
changes that account for decreased enzyme-substrate affinity appear to be nullified by
increased temperatures. The dissociation of the enzyme-product complex (k2 in
Equation 1-3, Chapter 1) is typically the limiting step in catalysis and is often referred to
as the apparent rate of catalysis. However, at 40 ˚C pressure affected the substrate
binding (k1/k-1 in Equation 1-3, or KM in Equation 1-4 Chapter 1), thus altering the
limiting step. The pressure dependence of the Michaelis Menten constant can be
determined and used to obtain the so-called reaction volume (ΔV KM) shown in equation
3-1 [28].
(3-1)
89
Pressure effects on substrate binding are thought to be the primary cause of pressure
sensitivity for several enzymatic reactions. According to Michels and Clark [28], the
ΔVKM can vary dramatically, and even change sign, depending on the substrate. In other
words, increasing pressure can increase or decrease the affinity of the substrate to the
enzyme. However, because an increased KM was only observed at 200 MPa and 40 ˚C,
the inhibitory effect of pressure on substrate binding may be overcome with elevated
temperature. Furthermore, since Vmax increased with pressure regardless of
temperature, any changes in substrate binding (KM) are overshadowed by increases in
rate of the limiting step (k2).
Several assumptions have been made to determine the KM and Vmax of lipase
catalyzed isoamyl acetate formation while in excess alcohol. These assumptions reduce
the Ping-Pong Bi Bi mechanism shown in Fig 3-1 to a simple one substrate one product
Michaelis Menten equation. It is assumed that alcohol-enzyme binding (KM2) is faster
than acid-enzyme binding (KM1) meaning that KM2 is not a limiting step. Therefore KM1 is
representative of the overall KM. It is also assumed that KM2 is not affected by the
concentration of acid. These assumptions reduce KM1 and KM2 to just KM. Furthermore, it
is assumed that the release of the ester (kcat2) is the overall slow/limiting rate and that
the release of water (kcat1) is not affected by the concentration of acid. Therefore kcat2 is
representative of the overall kcat (k2 from equation 1-3). Lastly, it is assumed that
isoamyl alcohol (as a substrate) provides no inhibitory action regardless of
concentration. These assumptions are not made arbitrarily. Evidence has been provided
that isoamyl alcohol has no inhibitory effects on lipase catalyzed synthesis of isoamyl
acetate, acetic acid is only inhibitory above 100 mM (this study used 60 mM), and that
90
lipase has a greater affinity for acetic acid than isoamyl alcohol [221]. These findings
confirmed the Ping-Pong Bi Bi mechanism shown in Fig 3-1, but did not address the
assumption that the release of the final product ester (kcat2) is the overall slow/limiting
rate. However, in a mono-phasic anhydrous solvent system such as hexane, it is
typically understood that water release occurs rapidly due to equilibrium effects and its
release does significantly affect enzyme conformation due to dilution effects.
Pressure effects on lipase catalyzed reactions have been previously discussed (in
chapter 2) and have elaborated on the complexities of explaining pressure induced
activation. Pressure induced changes in activity or stability are most likely attributed to
one or more of the following; 1) shifts in tertiary structure of the lipase (thus affecting
exposure to active site, stability characteristics, etc.), 2) changes in solvent polarity
(affecting lipase tertiary structure and/or flexibility), 3) changes in substrate or solvent
molar volume (thus affecting viscosity and substrate concentration, 4) changes in the
limiting step, and 5) changes in chemical equilibrium rates of the reaction. Although it is
not completely clear, changes in KM provide evidence that pressure induced activation
may be related to changes in the tertiary structure of the lipase and/or the limiting steps
of the reaction.
Conclusions
This study provides evidence that increasing pressure can inhibit substrate (acetic
acid) to enzyme binding (KM), while increasing temperature overcomes this effect by
increasing Vmax. It also provides evidence that pressure increases the reaction rate of
lipase differently depending on the temperature within a define pressure range. These
findings contribute to future optimization of isoamyl acetate production studies by
91
providing the framework for proper pressure-temperature combinations and substrate
concentrations.
Acknowledgments
This project was supported by a Research Innovation Grant from the University of
Florida Institute of Food and Agricultural Sciences.
Figure 3-1. Temperature (○) and pressure (▲) profiles using the “pressure-first” method at 80 ˚C and 400 MPa.
Figure 3-2. Kinetic mechanism (Ping Pong Bi Bi) of lipase-catalyzed synthesis of isoamyl acetate from acetic acid and isoamyl alcohol using Cleland’s notation where E represents free enzyme and E* is the activated enzyme state.
Ester
Alcohol
Water
Acid
E E∙Acid E*∙Water E*∙Alcohol
E∙Ester
E
KM1 kcat1 KM2 kcat2
92
Figure 3-3. Effect of pressure on Vmax at (●) 40 °C and (■) 80 °C for lipase-catalyzed production of isoamyl acetate (Novozyme 435 in n-hexane). Error bars represent standard error of the slope of apparent initial rate calculated from linear regression using a 95% confidence interval.
Figure 3-4. Linearized effect of pressure on V0 according to Eyring equation at (●) 40 and (■) 80 °C for lipase catalyzed production of isoamyl acetate.
93
Figure 3-5. Lineweaver-Burk plot of isoamyl acetate production at (♦) 0.1 MPa and 40 ˚C, (■) 200 MPa and 40 ˚C, (▲) 0.1 and 80 ˚C, and at (●) 200 MPa and 80 ˚C. Rate is expressed as mmol isoamyl acetate L-1 s-1 while substrate concentration is expressed as mmol L-1 acetic acid.
Table 3-1. Activation volume using the Eyring equation at 40 and 80 °C for lipase catalyzed production of isoamyl acetate. ± Values represent the standard error of the linear regression used in determination of activation volume.
Temperature Pressure ΔV‡
(cm3 mol-1) (˚C) (MPa)
40 1-100 -21.6 ± 2.9
80 10-125 -12.9 ± 1.7
Table 3-2. Michaelis-Menten kinetic parameters KM (mmol L-1) and Vmax (mmol L-1 s-1) of lipase catalyzed isoamyl acetate formation in hexane at 40 or 80 ˚C and 0.1 or 200 MPa. The ± values represent standard error from linear regression.
Temperature Pressure KM Vmax
(˚C) (MPa)
40 0.1 2.4 ± 0.004 7.7E-3 ± 2.0E-3
200 38.0 ± 0.684 7.3E-2 ± 1.8E-2
80 0.1 4.7 ± 0.094 4.3E-2 ± 2.0E-2
200 6.2 ± 1.303 4.2E-1 ± 2.1E-1
94
CHAPTER 4 ENHANCMENT OF NATURAL FLAVOR SYNTHESIS USING HIGH PRESSURE AND
AN IONIC LIQUID-ALCHOL BIPHASIC MEDIA
Introduction
Room temperature ionic liquids (ILs) are liquids that are composed completely of
ions and are liquid at or near room temperature [237]. They have garnered much recent
attention due to their unique properties as a reaction medium. They can have near-zero
vapor pressure (the pressure of a vapor in thermodynamic equilibrium with its
condensed phase), high thermal stability, and widely tunable properties (by changing
the cation/anion combination) such as polarity, hydrophobicity, and solvent miscibility
[237]. ILs are attractive reaction media because their use can enhance enzyme stability
[53, 54, 238, 239], selectivity [240], and reaction rates [238, 241]. Also, as compared to
mono-phasic systems, ILs utilized in a bi-phasic system can improve downstream
processing and separation operations when using free enzymes, thus improving
production efficiency [160, 237, 242]. Production efficiency is improved by helping
facilitate the physical separation of the reactant and product layer while leaving the
enzyme-IL layer unadulterated. Furthermore, enzymes in ILs have been termed as
“carrier-free” immobilized [243]. Like traditional carrier-bound immobilization, carrier-free
immobilization is also a method of modifying an enzyme to enable enzyme, solvent,
substrate, or product separations, extractions, or recycling to occur without loss of
enzyme activity. The main difference is that carrier-bound immobilization requires the
enzyme to be bound to a non-catalytic support while carrier-free does not. Types of
carrier-free immobilization include cross-liked enzyme crystals (CLECs), cross-linked
enzyme aggregates (CLEAs), and cross-linked dissolved enzymes (CLEs). Cao and
others [243] described how carrier-free immobilized enzymes generally exhibit 10-1000
95
times higher volumetric activity (U/g) versus carrier-bound. Carrier-free immobilized
CALB can also be used and recycled in both discontinuous [54] and continuous [244]
processes for ester synthesis with excellent operational stability, even under harsh
conditions (e.g. SC-CO2 at 150 ◦C and 10 MPa) [241, 245]. The combination of these
attributes along with the ease of recyclability (ability to easily separate using simple
decanting and purify using distillation techniques due to their high boiling point) add to
their growing application in diverse processes and make them useful alternatives to
organic solvents.
In an effort to determine the optimal IL for CALB synthesis, Lozano and others
[246] tested six different ILs. All the assayed ILs proved adequate media for enzyme-
catalyzed transesterification, and activity was increased with respect to that obtained in
organic solvents of similar polarity. For example, 1-ethyl-3-methylimidazolium
tetrafluoroborate enhanced 5- and 4-times the synthetic activity and half-life time
respectively of lipase in comparison to 1-butanol [246]. Lou and others [240] also found
that The IL 1-butyl-3-methylimidazolium tetrafluoroborate can serve as an excellent co-
solvent with buffer in place of traditional organic solvents for Novozym 435 mediated
hydrolysis of d,l-phenylglycine methyl ester with the advantage of markedly improved
enantioselectivity and activity.
ILs have been previously studied in combination with enzyme enhancement
techniques such as immobilization, microwave heating, and biphasic media. Combing
the use of ILs with different immobilizations resulted in increasing the half life of CALB
up to six-fold in hexane at 95 ˚C and increased synthetic activity up to six-fold in SC-
CO2 [158]. Combining microwave heating with 20 different ILs with different polarity,
96
viscosities, hydrophobicity, and water content revealed that IL stabilization and
activation effects on CALB were greatest with dried ILs and non-dried enzymes [247].
Using ILs in a bi-phasic media resulted in a stabilized CALB which allowed the enzyme
to be reused after 7-10 cycles with optimum conditions yielding nearly 100% isoamyl
acetate conversion [52]. Lastly, HHP stabilized and activated CALB (shown in chapter 2
and 3) in hexane. However, the effects of combining HHP and an IL-alcohol biphasic
system on any enzyme catalyzed reaction have yet to be documented.
The working hypothesis of this study is that HHP in an IL-alcohol biphasic system
can be used to increase the rate of free and immobilized lipase catalyzed isoamyl
acetate synthesis. The specific objectives are: 1) determine the production of isoamyl
acetate from isoamyl alcohol and acetic acid by free and immobilized lipase in an IL-
alcoholic biphasic system, 2) determine the effects of high pressure on the activation
energy of free lipase in an IL-alcoholic biphasic system, and 3) determine the effect of
temperature on the activation volume of free lipase in an IL-alcoholic biphasic system.
Materials and Methods
Materials
Enzyme and reagents
Lipases were from Candida antarctica lipase B (CALB) expressed in Aspergillus
oryzae and either immobilized on a macro porous acrylic resin (Novozyme 435® E.C.
3.1.1.3: 13.10 U/mg) or free (BioChemika # 65986: 1.51 U/mg) and obtained from
Sigma Aldrich (St. Louis, MO USA). Isoamyl alcohol, glacial acetic acid, hexane,
hexanol, toluene, and the ionic liquid 1-Butyl-3-methylimidazolium hexafluoro-phosphate
(bmimPF6) were obtained from Fisher Scientific (Pittsburg, PA USA). All solvents and
substrates were held at -10 °C or on ice while preparing for assay.
97
HHP system
The HHP system was from Unipress Equipment (Warsaw, Poland) and all other
auxiliary equipment and instrumentation was described in Chapter 2.
Methods
Reaction conditions
Enzyme was added (3.75 U/mL) into the reaction vial before adding isoamyl
alcohol (76.5% v/v), ionic liquid (bmimPF6, 13.0% v/v), glacial acetic acid (9.45% v/v),
toluene (as a internal standard, 0.39% v/v) and water (0.88% v/v), according to the
optimized proportions presented by Feher and others [52] for the same system. The
custom made reaction vial is depicted in Fig. 4-1and shown in Appendix B.The reaction
vial plunger was moved into position to eliminate air bubbles then sealed with a
Luer-lock™ plug. The reaction vial was then placed in the high pressure reaction
chamber being held at 5 °C. Polydimethylsiloxane silicone liquid (Accumetric, Inc.,
Elizabethtown, KY USA) was added as hydraulic fluid to fill the reactor. The reactor was
sealed and pressurized. After pressure reached the set-point, temperature was adjusted
to the set-point. Upon completion of incubation, the temperature was returned to 5 °C,
and the reactor was depressurized and opened. Adiabatic heating or cooling effects
associated with HHP systems upon pressurization and depressurization were not
significant factors because temperature controlled jacket limited temperature
fluctuations to less than 2 °C. Pressure and temperature had no effect on the reaction in
the absence of enzyme with or without presence of IL at pressures up to 400 MPa and
80 ˚C for 2.5 h (data not shown). Which was similar to previous studies [52, 224] where
isoamyl acetate production was negligible in absence of a catalyst. Samples were
treated and assayed in a randomized block design, blocked by temperature for
98
convenience, due to the time required to heat and cool water baths while pressure
selected randmoly.
Quantitative analysis
At selected incubation times, the reactor was cooled, depressurized and the
reaction vial was withdrawn. A 10-μL aliquot was drawn from the top (alcohol) phase
through the Luer-lock™ tip, diluted to 1 mL in hexane, and dried over excess
ammonium sulfate anhydrous and sodium bicarbonate to remove remaining acetic acid
and water. Then 10 μL of 7.9 X 10-5 mM hexanol in hexane was added as a second
internal standard in preparation for GC-FID analysis. The toluene standard was added
at the initiation of the reaction to account for error associated with transferring and
sample loss, while the hexanol internal standard added prior to GC-FID injection
accounts for error associated with the GC-FID analysis. Reaction progress was
monitored using GC-FID 5890 (HP, Palo Alto, CA USA) with a ZB-5 column (30 m
length × .53 mm ID × 1.5 μm thickness) at a gradient temperature from 50 ˚C to 90 °C at
5 ˚C min-1. Injector temperature was held at 200 ˚C and FID detector at 250 °C. Peak
identification and quantification was determined using pure standards and a calibration
curve. Linear regression analysis was conducted to generate apparent initial reaction
rates expressed as rate of isoamyl acetate formed per enzyme unit. Reaction
stoichiometry has been recently reviewed and confirmed [38, 42, 221] as shown in
equation 2-1, which allowed kinetic analysis to be conducted by following product
(isoamyl acetate) formation.
Conversion using free and immobilized lipase
Free or immobilized lipase was incubated at either 0.1 or 300 MPa for 3 h at 42,
63.5, or 80 ˚C. After incubation was complete the reaction vial was withdrawn and an
99
aliquot was analyzed as previously described. Reactions and analysis were conducted
in triplicate and error represented as standard deviation.
Activation energy
Free lipase was incubated at either 0.1 or 300 MPa at 40.0, 49.4, 59.0, 69.3, or
80.0 ˚C. At 30-min intervals the reaction mixture was cooled, depressurized, and
aliquots were taken and analyzed as described above to determine apparent initial rate.
Linear regression analysis was conducted using Excel (Microsoft Office 2007) data
analysis tool. Error was represented as standard error of the linear regression. Apparent
activation energy (Ea) was determined using the Arrhenius equation (shown in Equation
1-7, Chapter 1).
Activation volume
Free lipase was incubated at pressures from 0.1 to 500 MPa at 40 or 80 ˚C. At
30-min intervals the reaction mixture was cooled, depressurized, and aliquots were
taken and analyzed as described above to determine apparent initial rate. Linear
regression analysis was conducted using Excel (Microsoft Office 2007) data analysis.
Error is represented as standard error of the linear regression. Activation volume (ΔV‡)
was determined using Eyring equation (described in Equation 1-1, Chapter 1).
Ionic liquid recovery
After each reaction cycle, the biphasic mixture was decanted to separate the
alcoholic and IL phase containing the lipase. The lipase and ionic liquid was then filtered
through filter paper (type: P8) from Fisher Scientific (Pittsburg, PA USA) to remove
protein aggregates. Then, to remove trace volatiles the IL was held at 70 ˚C under
vacuum for 8 h.
100
Results and Discussion
Qualitative Observations
The biphasic system appeared to change depending on the incubation conditions.
As shown in Fig. 4-2A the native enzyme-IL mixture appears clear with yellow
suspended enzyme. As shown in Fig. 4-2B, after incubation at 0.1 MPa the enzyme
appears white and mostly accumulated at the IL-alcohol interface. Following
incubations between 100 and 300 MPa (Fig. 4-2C), the enzyme appeared to be in a
dispersed cloud above the IL-alcohol interface. After incubation at ≥400 MPa the
enzyme-IL mixture appeared to be a semi-solid white mass upon depressurization and
cooling (shown in Fig. 4-2D). After approximately 15 minutes at ambient pressure and
temperature all treatments appeared as Fig. 4-2B. The formation of the white mass was
also observed with just the pure ionic liquid (data not shown). It remains unclear when
this apparent phase change occurs; either during come-up, incubation, or come-down.
Further analysis utilizing a high pressure optical cell is needed to determine accurately
the conditions which induce this previously unseen phenomenon. This temporary
immobilization shown in Fig. 4-2D has not been previously described, and may be
useful in aiding the separation of phases between reaction cycles.
Conversion with Free and Immobilized Lipase
Increasing temperature increased the production of isoamyl acetate for both free
and immobilized lipase (which is within the linear range of conversion as shown in Fig 4-
3) as shown in Fig. 4-4 and Fig. 4-5. Production also increased at 300 MPa compared
to at 0.1 MPa reaching a maximum relative increase of 4.9-fold at 63.5 ˚C with free
lipase. Production was ~10-fold higher with free lipase compared to immobilized lipase.
Based on these findings, the rest of the experiments used free lipase instead of
101
immobilized lipase due to catalytic efficiency differences. Production may be higher with
free lipase due to increased substrate-active site collisions associated with free lipases
becoming more dispersed in the alcohol phase due to continuous stirring as discussed
below.
Conversion of isoamyl alcohol and acetic acid to isoamyl acetate was more
efficient in an IL-alcohol biphasic system than in the mono-phasic system used in
Chapter 2. The maximal concentration after 95% conversion was about 60 mM after 1 h
in hexane, while the maximal concentration after 95% conversion was about 1500 mM
after 4 h in the IL-alcohol biphasic system. Furthermore, catalysis in an IL-alcohol
biphasic system benefits from the advantage of potentially having an inhibitory
substrate, acetic acid, in a different phase than the enzyme, thus reducing substrate
inhibition [52]. For example, acetic acid was shown to have strong inhibitory effects on
lipase at concentrations as low as 0.1 M in hexane (increasing concentration from 0 to
0.1 M doubled the time required to reach full conversion) [221]. High concentration of
acetic acid may be affecting the pH of the aqueous mono-layer around the enzyme.
However, acetic acid concentration can be increased up to 3.6 M in a “solvent free”
(isoamyl alcohol based solvent) system before experiencing lipase inactivation [47].
Therefore, utilization of the IL-alcohol biphasic system benefits from the lipase being in
a separate phase than the acetic acid and from the increased allowable concentrations
of acetic acid due to being in the alcohol based “solvent free” system.
Determination of Activation Energy
Temperature effects on apparent initial rate are shown in Fig. 4-6 and transformed
into Arrhenius plots in Fig. 4-7. The apparent activation energy (Ea) derived from the
slope of the lines in Fig 4-7 is shown in Table 4-1. It is assumed that apparent initial
102
rates are representative of the actual initial rates. It is also assumed that the substrate
(acetic acid) is available to CALB in excess (KM << [S]). Although the KM of this reaction
has not been determined in this IL-biphasic mixture, it has been determined in
monophasic hexane in Chapter 3 to be from 2 to 38 mM (acetic acid) depending on the
reaction conditions. This reaction in the IL-alcoholic biphasic system utilized acetic acid
at 1589.5 mM which is much greater than the KM determined in hexane. Pressure only
affected the Ea of immobilized lipase (28% increase) which was similar to isoamyl
acetate synthesis catalyzed by CALB at HHP in hexane as discussed previously in
Chapters 2 and 3. The Ea values in Table 4-1 are higher than similar previous studies in
an IL-biphasic mixture (27.3 kJ mol-1) [52], in a solvent free system (28.7 kJ mol-1) [47],
and in hexane (35.7 to 47.8 kJ mol-1) at various pressures (from Chapter 2). With
regards to Ea in IL-biphasic mixture, differences may be attributed to use of different
temperatures, since this study examined 5 temperatures from 40 and 80 ˚C while Feher
and others [52] used only 4 temperatures between 30 and 60 ˚C with no mention of the
error. Likewise, Guvenc and other [47] only used 3 temperatures from 30 to 50 ˚C to
determine Ea with no mention of error. Finally, the Ea results from Chapter 2 in hexane
used the same lipase but it was immobilized, which may account for differences in Ea.
Unlike previous results in hexane (from Chapter 2), this study in IL-alcohol biphasic
system found a continual increase in reaction rates within the temperature range tested
(up to 80 ˚C) at all pressures tested. This may be attributed to the stabilization effects of
ionic liquid and/or high pressure on lipase. The possible mechanisms of pressure
induced stabilization have been previously described in Chapter 1 and 2. Although the
stabilization effects of ILs has yet to be fully understood, it is thought to be related to the
103
ILs ability to 1) negate substrate or product inhibitory action, 2) prevent essential water
loss associated with thermal denaturation as organic solvents do, 3) remove excess
water produced from esterification reactions also as organic solvents do, and 4) have
electrostatic interactions with the enzyme. Furthermore, Lozano and others [54]
suggested that since ILs form a strong ionic matrix, and added enzyme is considered
dispersed or included but not dissolved, an optimal microenvironment may be formed
for improved stability and activity. This last proposed mechanism is the most likely since
organic solvents also have interactions with substrates and/or products, restrict
essential water loss, facilitate excess water removal, and can have electrostatic
interactions with the enzyme but do not possess the ability to disperse an enzyme like
an IL. However, the activities are different when using the same enzyme and the same
reaction but changing the solvent system.
Determination of Activation Volume
As shown in Fig. 4-8, increasing pressure increased the apparent initial reaction
rate of free lipase at 40 and 80 ˚C from 0.1 to 500 MPa. It is assumed that apparent
initial rates are representative of the actual initial rates. It is also assumed that the
substrate (acetic acid) is available to CALB in excess (KM << [S]) for the reasons
previously discussed when describing the activation energy results. This reaction
utilized acetic acid at 1589.5 mM which is much greater than the KM determined in
hexane. Pressure effects resulted in a 15 and 25-fold increase in apparent initial rate
from 0.1 MPa to 500 MPa at 40 and 80 ˚C respectively. The activation volume (ΔV‡)
was -16.1 ± 1.5 and 16.7 ± 1.4 cm3 mol-1 at 40 and 80 ˚C respectively and was derived
from the slope of the plots shown in Figure 4-9. The ΔV‡ was negative and unchanged
by temperature, therefore increasing pressure continuously increased initial rates
104
regardless of temperature. These results are different than in chapter 3 where the
negative ΔV‡ of CALB catalyzed isoamyl acetate synthesis in hexane was decreased by
increasing temperature from -21.6 ± 2.9 at 40 ˚C to 12.9 ± 1.7 at 80 ˚C. This study found
a negative ΔV‡ throughout the entire pressure range tested (0.1 to 500 MPa). This is in
contrast to CALB in hexane from chapter 2 that found a negative ΔV‡ from 0.1 to 200
MPa (-21.6 and -12.9 at 40 and 80 ˚C respectively) and positive ΔV‡ from 300 to 500
MPa (14.3 and 15.2 at 40 and 80 ˚C respectively). These differences between
temperature affects on ΔV‡ indicate that the solvent (either hexane or IL) has an effect
on pressure induced activation.
Similarly, the activity and selectivity of free Candida antarctica lipase B (CALB)-
catalyzed trans-esterification of butyl butanoate (a flavor ester) were both higher in
water-immiscible but not water-miscible ionic liquids than in hexane [248]. This was
explained as being due to the increasing hydrophobicity of the IL involves a better
preservation of the essential water layer, reducing the direct protein-ion interactions.
Likewise, CALB increased activity in all four ILs tested in comparison with hexane and
1-butanol. Also, according to Lozano and others [54], the lipase was “over-stabilized” in
ionic liquids as evidenced when the reuse of free lipase in continuous operation cycles
showed a half-life time 2,300 times greater than that when the enzyme was incubated in
the absence of substrate, and had selectivity higher than 90%. Interestingly, IL
pretreated lipase also had higher activity and stability than untreated lipase for the
hydrolysis of p-nitrophenol butyrate in phosphate buffer. According to Nara and others
[238], pretreated lipase maintained activity after seven days at 60 ˚C in phosphate
buffer, while untreated lipase was fully inactivated after only 12 h at the same
105
conditions. It was suggested that this may be caused by the IL-coated lipase having
altered structure thus enhancing activity and stability of the lipase. More recently, Zhao
studied [247] microwave heating effects on CALB activity in twenty different ILs. Higher
activity was observed compared to conventional thermal heating and varied depending
on IL purity, polarity, hydrophobicity, and viscosity.
Besides conventional organic solvents or IL-alcohol biphasic mixtures,
compressed or supercritical fluids/gases have also been examined as solvents at
elevated pressures. CALB was shown to be effective at synthesizing isoamyl acetate in
SC-CO2 at higher initial reaction rates when compared to n-hexane while maintaining
activity from 8 to 30 MPa [161]. These results were explained as being due to increased
diffusivity of the reactants in the medium. In a similar study at 60 ˚C and 8 MPa in SC-
CO2, lipase activity increased 84-fold with respect to synthesis in organic solvents while
maintaining stability showing a 360 cycle half-life. Increased activity was explained as
improved micro-environments around the enzyme [108]. In another study,
Pseudomonas cepacia lipase (PCL) catalyzed transesterification of 1-phenylethanol
with vinyl acetate in SC-CO2 showed an increase in catalytic efficiency up to 15 MPa.
However, ΔV≠ did vary with pressure range used, reaching a maximum negative value
of -1340 cm3 mol-1 at 7.4 MPa [55]. High negative ΔV≠ would be expected in SC-CO2 at
this narrow pressure range (0.1–15 MPa) due to changes in solvent phase and density
as well as solubility and partitioning of substrates but not as direct effect on enzyme
activity.
106
The combination of IL and HHP may be altering the tertiary structure of the lipase,
thus activating and/or stabilizing the lipase. Stabilization allows the activation effects to
be observed at a wider temperature-pressure range.
Conclusions
This study has provided evidence that the conversion of isoamyl alcohol and
acetic acid to isoamyl acetate in an IL-alcoholic biphasic system is 10 times more
efficient with free than with immobilized lipase. Also rate of conversion was higher at
elevated pressure for both free and immobilized lipase. High pressure had no effect on
the apparent activation energy of free lipase and temperature had no effect on the
apparent activation volume, which was negative throughout the pressure range tested.
Lastly, the observation of a temporary immobilization of free lipase within the IL phase
provides new insight into a possible technique, such as rapid decanting, for improving
separation of the reactants and products from the IL-enzyme mixture.
Acknowledgements
This project was supported by a Research Innovation Grant from the University of
Florida Institute of Food and Agricultural Sciences.
107
Figure 4-1. Depiction of the custom made IL-HHP reaction vial.
Figure 4-2. Reaction vessels with ionic liquid biphasic mixture and free lipase.
108
Figure 4-3. Concentration (mM) of isoamyl acetate produced by CALB (7.5 U/ml) in an IL-alcohlic biphasic system at 40 ˚C. Error bars represent standard deviation of three replicates.
0
20
40
60
80
100
120
140
42 63 80
[Is
oa
my
l A
ce
tate
] (m
M)
Temperature (˚C)
Figure 4-4. Concentration (mM) of isoamyl acetate produced after 3 h incubation per unit enzyme of free CALB at (grey) 0.1 or (black) 300 MPa. Error bars represent standard deviation of three replicates.
109
0
2
4
6
8
10
12
42 63 80
[Is
oa
my
l A
ce
tate
] (m
M)
Temperature (˚C)
Figure 4-5. Concentration (mM) of isoamyl acetate produced after 3 h incubation per unit enzyme of immobilized CALB at (grey) 0.1 or (black) 300 MPa. Error bars represent standard deviation of three replicates.
Figure 4-6. Apparent initial rate per unit enzyme of free CALB at (○) 0.1 or (□) 300 MPa. Error bars represent standard error of linear regression.
110
Figure 4-7. Determination of activation energy using the Arrhenius equation at (◊) 0.1 and (□) 300 MPa.
Figure 4-8. Apparent initial rate per unit enzyme of free CALB at (○) 40 or (□) 80 ˚C. Error bars represent standard error of linear regression of five data points.
111
Figure 4-9. Determination of activation volume using the Eyring equation at (◊) 40 and (□) 80 °C.
Table 4-1. Activation energy (Ea) of free and immobilized lipase at 0.1 or 300 MPa
Pressure (MPa) Ea ± Std Error
Immobilized 0.1 43.4 ± 3.1
300 55.4 ± 0.1
Free 0.1 55.6 ± 4.2
300 56.2 ± 4.6
112
CHAPTER 5 IN-SITU ANALYSIS OF LIPASE STRUCTURAL CHANGES INDUCED BY HIGH
PRESSURE AND THERMAL TREATMENT
Introduction
High pressure (HP) affects proteins and enzymes by changing their structural
conformation which can be monitored using spectroscopic techniques. As discussed in
the previous chapters, pressure induced activation and stabilization may be related to
conformational changes in the enzyme structure. Currently, the effects of (HP) on
enzyme structure is scarce because there are few laboratories equipped with HP optical
cells coupled to the instrumentation necessary for such studies. Most conventional
methods of monitoring conformational changes in enzyme structure induced by HP
require ex situ measurements. While these studies are adequate for certain studies,
they provide no insight into the continuous conformational changes that occur during
each sequence of heating, pressurization, hold time, cooling, and depressurization.
Lastly, the protein/enzyme may be reversibly denatured depending on the conditions;
therefore observations conducted after a treatment at ambient conditions would be less
than accurate.
Some conformational studies have been conducted in situ at elevated pressure
using various other technique such as; Raman spectroscopy [201, 249], Fourier
transmission [250], nuclear magnetic resonance (NMR) [251], X-ray scattering [228],
and second and fourth ultraviolet derivative spectroscopies [227, 252-255] have also
been developed for protein and/or enzyme analysis at HHP.
The objective of this study is to continuously measure in situ conformational
changes in lipase at HP. Achieving this objective will allow greater understanding of
113
conformational changes at elevated pressures which may by correlated to pressure
induced activation and stabilization.
Materials and Methods
Materials
Enzyme and reagents
Free lipase was from Candida antarctica lipase B (CALB) expressed in Aspergillus
oryzae and (BioChemika # 65986: 1.51 U/g) and obtained from Sigma Aldrich (St.
Louis, MO USA). Lipase was dissolved in a 20 mM sodium phosphate-dibasic buffer pH
7 at a concentration of 20 U/mL and stored at 5 ˚C. Polydimethylsiloxane silicone liquid
(Accumetric, Inc., Elizabethtown, KY USA) was added as hydraulic fluid to fill the high
pressure reactor.
Fiber optic spectrometer
Spectral analysis is achieved with a USB 2.0 Fiber Optic Spectrometer (Model
USB4000) controlled and monitored by OOIBase 32 spectrometer operating software
and connected by 600 μm core diameter fibers (model QBIF600-VIS/NIR) all from
Ocean Optics (Dunedin, Fl). The UV-Vis-near IR light source is a Deuterium-Halogen
light (model DH-2000) from Mikropack (Ostfildern Germany).
High pressure optical cell
Determination of structural changes in lipase at pressures up to 500 MPa is
achieved through use of a custom designed and manufactured HP cell. The HP optical
cell and connections is depicted in Fig 5-1 and a picture is shown in Appendix C. It has
3 sapphire optical windows at 90 and 180˚ angles which allow monitoring of a small
sample (~2 mL) though fluorescence spectroscopy. The HHP optical cell is pressurized
and temperature controlled by a HHP micropump (model MP5), and a pump controller
114
(MP5 micropump control unit) all from Unipress Equipment (Warsaw, Poland). The
optical cell is temperature-controlled with a water jacket alternatively fed by two water
baths (Isotemp 3016D); one cooling (10 °C ± 0.1 °C) and another heating (80 °C ± 0.1
°C) from Fisher Scientific and controlled by an array of pinch valves. The optical HHP
cell is comprised of stainless steel and CuBe alloy and has connections for
thermocouples.
In-Situ optical analysis
Fluorescence emission spectra is recorded continuously in situ with an excitation of
285 nm and scanned at a right angle in the emission range of 250-500 nm while
recording at 350nm (the specific wavelength of tryptophan) according to a previous
study [169]. Changes in tryptophan residues are observed as they shift from buried
inside the enzyme (native) to exposed on the surface (denatured) or vice versa.
Changes in fluorescence of buffer as well as pressurization fluid are negligible as
determined by monitoring fluorescence changes in the absence of enzyme. A
continuous flow of nitrogen blanketed the sapphire windows to prevent moisture
condensation upon cooling. After insertion of the sample cuvette, the reactor was
sealed and pressurized. After pressure reached 500 MPa, temperature was adjusted to
80 ˚C using the pressure-first method discussed in Chapter 2. Upon completion of the
incubation time, the reactor was cooled to 10 ˚C and depressurized to 0.1 MPa. This
heating and pressurization sequence was repeated with continuous fluorescence
monitoring to observe cycling effects. Adiabatic heating or cooling effects commonly
associated with HHP systems upon pressurization and depressurization were not
significant factors as the temperature controlled jacket limited temperature fluctuations
to less than 2 °C.
115
Results and Discussion
The results of continuous monitoring of fluorescence at 350 nm are shown in Fig.
5-2. Fluorescence intensity (indicative of tryptophan exposure) changed depending on
the applied pressure and temperature combination as well as the number of previous
cycles. Upon initial pressurization the fluorescence intensity decreases then recovers
slightly after reaching 500 MPa. With increasing temperature the fluorescence intensity
increased. During incubation the intensity remained constant or slightly decreased
before decreasing during cooling. After depressurization the intensity decreases again
to reach a value lower than prior to treatment. This general trend is repeated with each
cycle although the magnitude of change is lessened. These results indicate that lipase
conformation is altered depending on the temperature-pressure combination, which
offers a possible explanation to pressure induced activation and/or stabilization.
However, the scattering effects associated with enzyme denaturation and aggregations
have not been accounted for.
In a similar study, the effects of incubating Rhizomucor miehei lipase at
temperatures from 40 to 60 ˚C and 0.1 MPa or at pressures from 300 to 500 MPa at 25
˚C was observed using fluorescence spectroscopy ex situ [169]. Results suggested that
the conformational changes induced by pressure were different from those induced by
temperature, which in agreement with the findings in Fig. 5-1. In contrast, no significant
shift in the 350 nm band was observed for thermal treatment, which is different than
found in this study.
According to the previous results discussed in Chapters 2 and 3 activity is higher
at elevated pressure-temperature combinations and according to the results shown in
Fig 5-1 tryptophan fluorescence is also increased at elevated temperature-pressure
116
combinations. Therefore, there may be a correlation between pressure induced
activation and pressure induced conformational changes. This is in agreement with Noel
and others [169] who found that the intensity of lipase tryptophan fluorescence
decreased with a corresponding decrease in activity. In other words, a 63% decrease in
relative fluorescence corresponded to an 80% reduction in relative residual activity.
However, a direct comparison between results is difficult due to differences in lipase,
pressure-temperature combinations, and measuring in situ versus ex situ.
Conclusions
Fluorescence spectroscopy of lipase has been conducted continuously in situ at
pressures up to 500 MPa and up to 80 ˚C. Results indicate immediate and profound
changes in tryptophan fluorescence as indicated by changes in the intensity at 350nm.
Evidence has been provided for a possible link between pressure induced activation
and pressure induced conformational changes. Although these results are qualitative,
they do provide a valuable insight into the conditions which trigger conformational
changes.
Acknowledgements
This project was supported by a Research Innovation Grant from the University of
Florida Institute of Food and Agricultural Sciences
117
Figure 5-1. Schematic representation of the high pressure optical cell with sapphire windows and fiber optic ports for continuous optical measurements in situ.
118
Figure 5-2. Intensity expressed in counts of fluorescence at 350 nm emitted from lipase during 3 cycles of pressurization (0.1 to 500 MPa), heating (10 ˚C to 80 ˚C), and 2 minute incubations followed by cooling and depressurization.
119
CHAPTER 6 COMPREHENSIVE RESULTS, DISCUSSION, AND FUTURE STUDIES
This research has filled various gaps in knowledge. The first chapter provided
evidence that high pressure stabilization and activation is not an isolated phenomenon
and occurs in many different enzymes, from different sources, in different
solvents/media, and with different optimal conditions. These findings are important
because they provide a base of evidence which can be used to further explore the
application of high pressure to improve enzyme catalysis. Since most enzymes
discussed are used in the food industry, there remains a gap in knowledge with regards
to enzymes from other industries. This has yet to be explored because high pressure
processing is a relatively new technology which has not be widely implemented in other
production processes. To fill this gap in knowledge, a broad sampling of enzymes
should be conducted from other industries (i.e. pharmaceutical industry) and studied
with regards to their pressure induced stabilization or activation properties.
Also in the first chapter, the possible mechanisms of pressure induced stabilization
and activation were compiled and discussed. Although several studies have alluded to
possible mechanisms, this was the first to comprehensively describe them and the data
behind these proposed mechanisms. By fully understanding the current state of
knowledge, future studies can be executed to explore the validity of these proposed
mechanisms, which will allow for better utilization of pressure-temperature
combinations.
The second and third chapters provided evidence that HHP can stabilize and
activate (up to 152% and 239% respectively) an immobilized lipase used to catalyze the
synthesis of isoamyl acetate in hexane. The gap in knowledge was filled by
120
determination of several parameters; including ΔV‡, Ea, Vmax, and KM while also
observing the effects of HHP on the immobilization support. This study was important
because it was the first to demonstrate pressure induced enhancement of the most
widely used enzyme (in synthesis reactions) in the most commonly used solvent
(hexane) for the production of a widely used product (isoamyl acetate). As a model
system, this study provides evidence of a new method to increase lipase activity and
stability that can be implemented in combination with existing enhancement techniques
such as immobilization, genetic engineered enzymes, and non-aqueous solvents.
However, several important questions remain unanswered. They include; what are the
mechanisms associated with pressure induced changes on reaction rate and substrate-
enzyme binding, what is the effect of temperature on ΔV‡ and ΔV KM, and what are the
long term effects on lipase stability and activity caused by HHP and high temperature
cycling. These questions remain unanswered due to lack of adequate time and proper
equipment. To explore mechanisms, a high pressure optical cell coupled to an
instrument capable of monitoring specific conformational changes (e.g. circular
dichroism) is required. Furthermore, a lipase that is soluble in a non-aqueous and non-
polar medium must be developed to adequately describe conformational changes
associated with increased activity and stability in hexane. To determine the effect of
temperature on ΔV‡ and ΔV KM a series of assays are needed at a range of
temperatures and pressures. Lastly, cycling effects over time can be determined by
repeated pressurizing, heating, cooling, and depressurizing until significant activity is
lost. Cycling studies can be conducted more efficiently by using a multi-cell high
pressure reactor. When these studies are complete and with the growing use of high
121
pressure processing driving the advancement of high pressure equipment and
processing technologies, the industrial commercialization of this HHP technique will be
a more feasible option for enzyme catalysis.
The fourth chapter demonstrated the activation effect (up to 25-fold activity
increase) of HHP on immobilized and free lipase used to catalyze synthesis of isoamyl
acetate in an ionic liquid-alcoholic biphasic mixture. The effects of HHP on lipase
activity were unknown in an ionic liquid-alcoholic biphasic mixture as no studies had
been done with any enzyme at HHP in this solvent system. This gap in knowledge was
achieved by the determination of both ΔV‡, Ea of lipase catalyzed isoamyl acetate
synthesis. These findings are important because they show how other solvent systems
(besides mono-phasic organic) can also be used in combination with HHP.
Furthermore, they demonstrated that free lipase is better suited than immobilized lipase
in this system which will allow future studies to proceed more effectively. Lastly, the
observation of the temporary immobilization phenomenon is a new and previously
undocumented occurrence. This unique phenomenon may aid in recycling during a
batch process by increasing the ease of decanting procedures while minimizing enzyme
and IL loss. The remaining gaps in knowledge include; how HHP and thermal treatment
cycling affect enzyme activity and stability, what is the best method of recycling the IL
while ensuring complete removal of dispersed lipase, and when does the temporary
immobilization phenomenon occur, how does it affect activity or stability, and how can it
be utilized to improve the reaction processing/recycling in a batch or semi-continuous
system. These questions remain unanswered due to time constraints, but can be readily
answered using currently available methods and equipment.
122
Lastly, in the fifth chapter a relationship between pressure-temperature induced
lipase activation and conformational changes was established. It was previously
unknown if HHP induced activation and stabilization was directly related to
conformational changes. These findings are important because they provide evidence
that HHP has direct effects on the catalyst (lipase) aside from any effect on the
chemical reaction, solvent, substrate, etc. With this evidence further studies can explore
precisely what changes are occurring in the lipase that account for increased activity
and stability. These needed studies were not conducted due to lack of proper spectral
monitoring equipment.
Although this research has filled some gaps in knowledge, much remains
unanswered. Further research is needed in using high pressure technology for more
cost-effective synthesis reactions such as the production of high value pharmaceuticals.
Cost-effectives can also be improved through the development of a continuous high
pressure reactor. Also, the optimization of enzyme catalysis in environmentally friendly
solvents such as ILs may reduce or eliminate the need for using toxic and flammable
organic solvents. Furthermore, if conformational studies can determine specific
structural changes that account for activation and stabilization then techniques such as
site-directed mutagenesis and site-specific immobilization may be applied to generate
similar conformational changes with similar activity and stability while at ambient
pressure.
123
APPENDIX A PICTURE OF HIGH HYDROSTATIC PRESSURE SYSTEM
124
APPENDIX B PICTURE OF HIGH HYDROSTATIC PRESSURE IONIC LIQUID REACTION VIAL
125
APPENDIX C PICTURE OF HIGH HYDROSTATIC PRESSURE OPTICAL CELL
LIST OF REFERENCES
[1] Zobell CE, Johnson FH. The influence of hydrostatic pressure on the growth and viability of terrestrial and marine bacteria. J Bacteriol 1949;57:179-189.
[2] Zobell CE, Morita RY. Barophilic bacteria in some deep sea sediments. J
Bacteriol 1957;73:563-568. [3] Fiebig J, Woodland AB, Spangenberg J, Oschmann W. Natural evidence for
rapid abiogenic hydrothermal generation of CH4. Geochim Cosmochim Acta 2007;71:3028-3039.
[4] Abe F, Horikoshi K. The biotechnological potential of piezophiles. Trends
Biotechnol 2001;19:102-108. [5] Certes A. Sur la culture, a l'abri des germes atmospheiriques, des eaux et des
sediments rapporteo par lea expeditions du ' Travailleur' et du ' Talisman,' 1882-83. C R Acad Sci Paris 1884;xcviii:pp. 690-693.
[6] Certes A. De l'action des hautes pressions sur les phenomenes de la
putrefaction et sur la vitalite des micro-organismes d'eau douce et d'eau de mer. C R Acad Sci 1884;xcix:pp. 385-388.
[7] Bridgman PW. The coagulation of albumen by pressure. J Biol Chem
1914;19:511-512. [8] Tewari G, Jayas DS, Holley RA. High pressure processing of foods: an overview.
Sci Aliment 1999;19:619-661. [9] Michels PC, Hei D, Clark DS. Pressure effects on enzyme activity and stability at
high temperatures. Adv Protein Chem 1996;48:341-376. [10] Cheftel JC. Review: High-pressure, microbial inactivation and food preservation.
Food Sci Technol Int 1995;1:75-90. [11] Guerrero-Beltran JA, Barbosa-Canovas G, Swanson BG. High hydrostatic
pressure processing of fruit and vegetable products. Food Rev Int 2005;21:411-425.
[12] Raso J, Barbosa-Canovas GV. Nonthermal preservation of foods using
combined processing techniques. Crit Rev Food Sci Nutr 2003;43:265-285. [13] Ludikhuyze L, Van Loey A, Indrawati, Smout C, Hendrickx M. Effects of
combined pressure and temperature on enzymes related to quality of fruits and vegetables: From kinetic information to process engineering aspects. Crit Rev Food Sci Nutr 2003;43:527-586.
[14] San Martin MF, Barbosa-Canovas GV, Swanson BG. Food processing by high hydrostatic pressure. Crit Rev Food Sci Nutr 2002;42:627-645.
[15] Northrop DB. Effects of high pressure on enzymatic activity. BBA-Protein Struct
M 2002;1595:71-79. [16] Mozhaev VV, Heremans K, Frank J, Masson P, Balny C. Exploiting the effects of
high hydrostatic-pressure in biotechnological applications. Trends Biotechnol 1994;12:493-501.
[17] Balny C, Mozhaev VV, Lange R. Hydrostatic pressure and proteins: Basic
concepts and new data. Comp Biochem Phys A 1997;116:299-304. [18] Mozhaev VV, Heremans K, Frank J, Masson P, Balny C. High pressure effects
on protein structure and function. Prot Struc Func and Gen 1996;24:81-91. [19] Sun MMC, Clark DS. Pressure effects on activity and stability of
hyperthermophilic enzymes. Hyperthermophilic Enzymes, Pt C, vol. 334, 2001, pp. 316-327.
[20] Michels PC, Clark DS. Pressure-enhanced activity and stability of a
hyperthermophilic protease from a deep-sea methanogen. Appl Environ Microbiol 1997;63:3985-3991.
[21] Summit M, Scott B, Nielson K, Mathur E, Baross J. Pressure enhances thermal
stability of DNA polymerase from three thermophilic organisms. Extremophiles 1998;2:339-345.
[22] Demirjian DC, Moris-Varas F, Cassidy CS. Enzymes from extremophiles. Curr
Opin Chem Biol 2001;5:144-151. [23] Gomes J, Steiner W. The biocatalytic potential of extremophiles and
extremozymes. Food Technol Biotech 2004;42:223-235. [24] Sellek GA, Chaudhuri JB. Biocatalysis in organic media using enzymes from
extremophiles. Enzyme Microb Tech 1999;25:471-482. [25] Morawski P, Coutinho JAP, Domanska U. High pressure (solid + liquid) equilibria
of n-alkane mixtures: experimental results, correlation and prediction. Fluid Phase Equilib 2005;230:72-80.
[26] Saiz AH, Mingo ST, Balda FP, Samson CT. Advances in design for successful
commercial high pressure food processing. Food Aust 2008;60:154-156. [27] Balasubramaniam B, Farakas D, Turek EJ. Preserving foods through high
pressure processing. Food Technol-Chicago 2008;11.08:32-38.
[28] Michels PC, Clark DS. Pressure-dependence of enzyme catalysis ACS Sym Ser
1992;498:108-121. [29] Balny C, Masson P. Effects of high-pressure on proteins. Food Rev Int
1993;9:611-628. [30] Gross M, Jaenicke R. Proteins under pressure- the influence of high hydrostatic-
pressure on structure, function, and assembly of proteins and protein compleses. Eur J Biochem 1994;221:617-630.
[31] Balny C. What lies in the future of high-pressure bioscience? BBA-Protein Struct
M 2006;1764:632-639. [32] Morild E. The theory of pressure effects on enzymes. Adv Protein Chem
1981;34:93-166. [33] Villeneuve P, Muderhwa JM, Graille J, Haas MJ. Customizing lipases for
biocatalysis: a survey of chemical, physical and molecular biological approaches. J Mol Catal B: Enzym 2000;9:113-148.
[34] Wilson L, Palomo JM, Fernández-Lorente G, Illanes A, Guisán JM, Fernández-
Lafuente R. Improvement of the functional properties of a thermostable lipase from alcaligenes sp. via strong adsorption on hydrophobic supports. Enzyme Microb Tech 2006;38:975-980.
[35] Mateo C, Palomo JM, Fernandez-Lorente G, Guisan JM, Fernandez-Lafuente R.
Improvement of enzyme activity, stability and selectivity via immobilization techniques. Enzyme Microb Tech 2007;40:1451-1463.
[36] Fernandez-Lafuente R, Cowan DA, Wood ANP. Hyperstabilization of a
thermophilic esterase by multipoint covalent attachment. Enzyme Microb Tech 1995;17:366-372.
[37] Guisan JM, Bastida A, Cuesta C, Fernandezlafuente R, Rosell CM.
Immobilization stabilization of alpha-chymotrypsin by covalent attachement to aldehydre agarose gels. Biotechnol Bioeng 1991;38:1144-1152.
[38] Romero MD, Calvo L, Alba C, Daneshfar A, Ghaziaskar HS. Enzymatic synthesis
of isoamyl acetate with immobilized Candida antarctica lipase in n-hexane. Enzyme Microb Tech 2005;37:42-48.
[39] Klibanov AM. Enzyme-Catalyzed Processes in Organic-Solvents. Ann N Y Acad
Sci 1987;501:129-129.
[40] Zaks A, Klibanov AM. Enzyme-Catalyzed Processes in Organic-Solvents. Proc Natl Acad Sci U S A 1985;82:3192-3196.
[41] Klibanov AM. Enzymatic catalysis in anhydrous organic solvents. Trends
Biochem Sci 1989;14:141-144. [42] Guvenc A, Kapucu N, Bayraktar E, Mehmetoglu U. Optimization of the enzymatic
production of isoamyl acetate with Novozym 435 from Candida antarctica. Chem Eng Comm 2003;190:948-961.
[43] Chang C-S, Wu P-L. Synthesis of triglycerides of phenylalkanoic acids by lipase-
catalyzed esterification in a solvent-free system. J Biotechnol 2007;127:694-702. [44] Karra-Chaabouni M, Ghamgui H, Bezzine S, Rekik A, Gargouri Y. Production of
flavour esters by immobilized Staphylococcus simulans lipase in a solvent-free system. Process Biochem 2006;41:1692-1698.
[45] Ghamgui H, Karra-Chaabouni M, Bezzine S, Miled N, Gargouri Y. Production of
isoamyl acetate with immobilized Staphylococcus simulans lipase in a solvent-free system. Enzyme Microb Tech 2006;38:788-794.
[46] Chang SW, Shaw JF, Shieh CH, Shieh CJ. Optimal formation of hexyl laurate by
Lipozyme IM-77 in solvent-free system. J Agric Food Chem 2006;54:7125-7129. [47] Guvenc A, Kapucu N, Mehmetoglu U. The production of isoamyl acetate using
immobilized lipases in a solvent-free system. Process Biochem 2002;38:379-386. [48] Shimada Y, Hirota Y, Baba T, Kato S, Sugihara A, Moriyama S, Tominaga Y,
Terai T. Enzymatic synthesis of L-menthyl esters in organic solvent-free system. J Am Oil Chem Soc 1999;76:1139-1142.
[49] Vija H, Telling A, Tougu V. Lipase-catalysed esterification in supercritical carbon
dioxide and in hexane. Bioorg Med Chem Lett 1997;7:259-262. [50] Knez Z, Habulin M, Primozic M. Enzymatic reactions in dense gases. Biochem
Eng J 2005;27:120-126. [51] Knez Z, Habulin M, Krmelj V. Enzyme catalyzed reactions in dense gases. J
Supercrit Fluid 1998;14:17-29. [52] Feher E, Illeova V, Kelemen-Horvath I, Belafi-Bako K, Polakovic M, Gubicza L.
Enzymatic production of isoamyl acetate in an ionic liquid-alcohol biphasic system. J Mol Catal B: Enzym 2008;50:28-32.
[53] Feher E, Major B, Belafi-Bako K, Gubicza L. On the background of enhanced stability and reusability of enzymes in ionic liquids. Biochem Soc Trans 2007;35:1624-1627.
[54] Lozano P, De Diego T, Carrie D, Vaultier M, Iborra JL. Over-stabilization of
Candida antarctica lipase B by ionic liquids in ester synthesis. Biotechnol Lett 2001;23:1529-1533.
[55] Celia E, Cernia E, Palocci C, Soro S, Turchet T. Tuning Pseudomonas cepacea
lipase (PCL) activity in supercritical fluids. J Supercrit Fluid 2005;33:193-199. [56] Penniston JT. High hydrostatic pressure and enzymic activity: Inhibition of
multimeric enzymes by dissociation. Arch Biochem Biophys 1971;142:322-332. [57] Eyring H, Magee JL. Application of the theory of absolute reaction rates to
bacterial luminescence. Journal of Cellular and Comparative Physiology 1942;20:169-177.
[58] Jiang B, Wang H, Li ZY. The use of biocatalysis for the production of flavours
and fragrances. Chinese J Org Chem 2007;27:377-384. [59] Gotor V. Biocatalysis applied to the preparation of pharmaceuticals. Org Process
Res Dev 2002;6:420-426. [60] Klibanov AM. Improving enzymes by using them in organic solvents. Nature
2001;409:241-246. [61] Berglund P. Controlling lipase enantioselectivity for organic synthesis. Biomol
Eng 2001;18:13-22. [62] Ke T, Klibanov AM. On enzymatic activity in organic solvents as a function of
enzyme history. Biotechnol Bioeng 1998;57:746-750. [63] Volkin DB, Staubli A, Langer R, Klibanov AM. Enzyme Thermoinactivation in
Anhydrous Organic-Solvents. Biotechnol Bioeng 1991;37:843-853. [64] Zaks A, Klibanov AM. The effect of water on enzyme action in organic media. J
Biol Chem 1988;263:8017-8021. [65] Klibanov AM, Cambou B, Zaks A. Enzyme-Catalyzed Processes in Organic
Media at 100-Degrees-C. Abstracts of Papers of the American Chemical Society 1984;188:29-MBTD.
[66] Rai N, Siepmann JI, Schultz NE, Ross RB. Pressure dependence of the
hildebrand solubility parameter and the internal pressure: Monte Carlo
simulations for external pressures up to 300 MPa. J Phys Chem C 2007;111:15634-15641.
[67] Krishna SH, Divakar S, Prapulla SG, Karanth NG. Enzymatic synthesis of
isoamyl acetate using immobilized lipase from Rhizomucor miehei. J Biotechnol 2001;87:193-201.
[68] Trodler P, Pleiss J. Modeling structure and flexibility of Candida antarctica lipase
B in organic solvents. BMC Struct Biol 2008;8:1-10. [69] Vulfson EN. Enzymatic synthesis of food ingredients in low-water media. Trends
Food Sci Tech 1993;4:209-215. [70] Adekoya OA, Sylte I. The Thermolysin Family (M4) of Enzymes: Therapeutic and
Biotechnological Potential. Chem Biol Drug Des 2009;73:7-16. [71] Torres S, Martinez MA, Pandey A, Castro GR. An organic-solvent-tolerant
esterase from thermophilic Bacillus licheniformis S-86. Bioresource Technol 2009;100:896-902.
[72] Dastoli FR, Musto NA, Price S. Reactivity of active sites of chymotrypsin
suspended in an organic medium. Arch Biochem Biophys 1966;115:44-48. [73] Zaks A, Klibanov AM. Enzymatic catalysis in nonaqueous solvents. J Biol Chem
1988;263:3194-3201. [74] Dastoli FR, Price S. Further studies on xanthine oxidase in nonpolar media. Arch
Biochem Biophys 1967;122:289-306. [75] Dastoli FR, Price S. Catalysis by xanthine oxidase suspended in organic media.
Arch Biochem Biophys 1967;118:163-165. [76] Klibanov AM. Enzymes that work in organic solvents. Chemtech 1986;16:354-
359. [77] Hoellrigl V, Hollmann F, Kleeb AC, Buehler K, Schmid A. TADH, the
thermostable alcohol dehydrogenase from Thermus sp ATN1: a versatile new biocatalyst for organic synthesis. Appl Microbiol Biotechnol 2008;81:263-273.
[78] Dordick JS, Isermann HP. Rules for Optimization of Biocatalysis in Organic
Solvents Introduction. Biotechnol Bioeng 2009;102:1-1. [79] Lee YS, Hong JH, Jeon NY, Won K, Kim BT. Highly enantioselective acylation of
rac-alkyl lactates using Candida antarctica lipase B. Org Process Res Dev 2004;8:948-951.
[80] Degn P, Zimmermann W. Optimization of carbohydrate fatty acid ester synthesis in organic media by a lipase from Candida antarctica. Biotechnol Bioeng 2001;74:483-491.
[81] Kirchner G, Scollar MP, Klibanov AM. Resolution of racemic mixtures via lipase
catalysis in organic solvents. J Am Chem Soc 1985;107:7072-7076. [82] Sun MMC, Tolliday N, Vetriani C, Robb FT, Clark DS. Pressure-induced
thermostabilization of glutamate dehydrogenase from the hyperthermophile Pyrococcus furiosus. Protein Sci 1999;8:1056-1063.
[83] Dallet S, Legoy M-D. Hydrostatic pressure induces conformational and catalytic
changes on two alcohol dehydrogenases but no oligomeric dissociation. Biochim Biophys Acta 1996;1294:15-24.
[84] Cho YK, Northrop DB. Effects of pressure on the kinetics of capture by yeast
alcohol dehydrogenase. Biochemistry-US 1999;38:7470-7475. [85] Morita RY, Haight RD. Malic dehydrogenase activity at 101 C under hydrostatic
pressure. J Bacteriol 1962;83:1341-1346. [86] Hei DJ, Clark DS. Pressure stablilization of proteins from extreme thermophiles.
Appl Environ Microbiol 1994;60:932-939. [87] Miller JF, Nelson CM, Ludlow JM, Shah NN, Clark DS. High pressure-
temperature bioreactor- Assays of thermostable hydrogenase with fiber optics. Biotechnol Bioeng 1989;34:1015-1021.
[88] Garcia-Palazon A, Suthanthangjai W, Kajda P, Zabetakis I. The effects of high
hydrostatic pressure on [beta]-glucosidase, peroxidase and polyphenoloxidase in red raspberry (Rubus idaeus) and strawberry (Fragaria × ananassa). Food Chem 2004;88:7-10.
[89] Indrawati, Van Loey AM, Ludikhuyze LR, Hendrickx ME. Pressure-temperature
inactivation of lipoxygenase in green peas (Pisum sativum): A kinetic study. J Food Sci 2001;66:686-693.
[90] Tedjo W, Eshtiaghi MN, Knorr D. Impact of supercritical carbon dioxide and high
pressure on lipoxygenase and peroxidase activity. J Food Sci 2000;65:1284-1287.
[91] Weemaes CA, Ludikhuyze LR, Van den Broeck I, Hendrickx ME. Kinetics of
combined pressure-temperature inactivation of avocado polyphenoloxidase. Biotechnol Bioeng 1998;60:292-300.
[92] Butz P, Koller WD, Tauscher B, Wolf S. Ultra-high pressure processing of onions - chemical and sensory changes. Food Sci Technol-Leb 1994;27:463-467.
[93] Gomes MRA, Ledward DA. Effect of high-pressure treatment on the activity of
some polyphenoloxidases. Food Chem 1996;56:1-5. [94] Crelier S, Robert MC, Claude J, Juillerat MA. Tomato (Lycopersicon esculentum)
pectin methylesterase and polygalacturonase behaviors regarding heat- and pressure-induced inactivation. J Agric Food Chem 2001;49:5566-5575.
[95] Anese M, Nicoli MC, Dallaglio G, Lerici CR. Effect of high-pressure treatments on
peroxidase and polyphenoloxidase activities. J Food Biochem 1995;18:285-293. [96] Rapeanu G, Van Loey A, Smout C, Hendrickx M. Thermal and high-pressure
inactivation kinetics of polyphenol oxidase in victoria grape must. J Agric Food Chem 2005;53:2988-2994.
[97] Dirix C, Duvetter T, Van Loey A, Hendrickx M, Heremans K. The in situ
observation of the temperature and pressure stability of recombinant Aspergillus aculeatus pectin methylesterase with Fourier transform IR spectroscopy reveals an unusual pressure stability of beta-helices. Biochem J 2005;392:565-571.
[98] Duvetter T, Fraeye I, Sila DN, Verlent I, Smout C, Clynen E, Schoofs L, Schols
H, Hendrickx M, Loey A. Effect of temperature and high pressure on the activity and mode of action of fungal pectin methyl esterase. Biotechnol Prog 2006;22:1313-1320.
[99] Fraeye I, Duvetter T, Verlent I, Ndaka Sila D, Hendrickx M, Van Loey A.
Comparison of enzymatic de-esterification of strawberry and apple pectin at elevated pressure by fungal pectinmethylesterase. Innov Food Sci Emerg 2007;8:93-101.
[100] Van den Broeck I, Ludikhuyze LR, Van Loey AM, Hendrickx ME. Inactivation of
orange pectinesterase by combined high-pressure and -temperature treatments: A kinetic study. J Agric Food Chem 2000;48:1960-1970.
[101] Sila DN, Smout C, Satara Y, Truong V, Loey AV, Hendrickx M. Combined
thermal and high pressure effect on carrot pectinmethylesterase stability and catalytic activity. J Food Eng 2007;78:755-764.
[102] Ly-Nguyen B, Van Loey AM, Smout C, Ozcan SE, Fachin D, Verlent I, Truong
SV, Duvetter T, Hendrickx ME. Mild-heat and high-pressure inactivation of carrot pectin methylesterase: A kinetic study. J Food Sci 2003;68:1377-1383.
[103] Hsu K-C. Evaluation of processing qualities of tomato juice induced by thermal
and pressure processing. Food Sci Technol-Leb 2008;41:450-459.
[104] Knez Z, Laudani CG, Habulin M, Reverchon E. Exploiting the pressure effect on
lipase-catalyzed wax ester synthesis in dense carbon dioxide. Biotechnol Bioeng 2007;97:1366-1375.
[105] Noel M, Lozano P, Combes D. Polyhydric alcohol protective effect on
Rhizomucor miehei lipase deactivation enhanced by pressure and temperature treatment. Bioprocess and Biosystems Engineering 2005;27:375-380.
[106] Marie-Olive MN, Athes V, Combes D. Combined effects of pressure and
temperature on enzyme stability. High Press Res 2000;19:707-712. [107] Nagesha GK, Manohar B, Udaya Sankar K. Enzymatic esterification of free fatty
acids of hydrolyzed soy deodorizer distillate in supercritical carbon dioxide. J Supercrit Fluid 2004;32:137-145.
[108] Lozano P, Víllora G, Gómez D, Gayo AB, Sánchez-Conesa JA, Rubio M, Iborra
JL. Membrane reactor with immobilized Candida antarctica lipase B for ester synthesis in supercritical carbon dioxide. J Supercrit Fluid 2004;29:121-128.
[109] Habulin M, Knez Z. Activity and stability of lipases from different sources in
supercritical carbon dioxide and near-critical propane. J Chem Technol Biotechnol 2001;76:1260-1266.
[110] De Oliveira D, Feihrmann AC, Dariva C, Cunha AG, Bevilaqua JV, Destain J,
Oliveir JV, Freire DMG. Influence of compressed fluids treatment on the activity of Yarrowia lipolytica lipase. J Mol Catal B: Enzym 2006;39:117-123.
[111] Srivastava S, Modak J, Madras G. Enzymatic synthesis of flavors in supercritical
carbon dioxide. Industrial & Engineering Chemistry Research 2002;41:1940-1945.
[112] Millar DB, Grafius MA, Wild JR, Palmer DA. High pressure stabilization of
acetylcholinesterase sizeozymes against thermal denaturation. Biophys Chem 1974;2:189-192.
[113] Fachin D, Van Loey A, Indrawati L, Ludikhuyze L, Hendrickx M. Thermal and
high-pressure inactivation of tomato polygalacturonase: A kinetic study. J Food Sci 2002;67:1610-1615.
[114] Buckow R, Weiss U, Heinz V, Knorr D. Stability and catalytic activity of alpha-
amylase from barley malt at different pressure-temperature conditions. Biotechnology and Bioengineering 2007;97:1-11.
[115] Heinz V, Buckow R, Knorr D. Catalytic Activity of Beta-Amylase from Barley in
Different Pressure/Temperature Domains. Biotechnol Prog 2005;21:1632-1638.
[116] Buckow R, Heinz V, Knorr D. Effect of high hydrostatic pressure-temperature
combinations on the activity of beta-glucanase from barley malt. J I Brewing 2005;111:282-289.
[117] Buckow R, Heinz V, Knorr D. Two Fractional Model for Evaluating the Activity of
Glucoamylase from Aspergillus Niger Under Combined Pressure and Temperature Conditions. Food Bioprod Process 2005;83:220-228.
[118] Athes V, Degraeve P, CavailleLefebvre D, Espeillac S, Lemay P, Combes D.
Increased thermostability of three mesophilic beta-galactosidases under high pressure. Biotechnol Lett 1997;19:273-276.
[119] Marques J, Vila-Real HJ, Alfaia AJ, Ribeiro MHL. Modelling of the high pressure-
temperature effects on naringin hydrolysis based on response surface methodology. Food Chem 2007;105:504-510.
[120] Pedro HAL, Alfaia AJ, Marques J, Vila-Real HJ, Calado A, Ribeiro MHL. Design
of an immobilized enzyme system for naringin hydrolysis at high-pressure. Enzyme Microb Tech 2007;40:442-446.
[121] Real HJV, Alfaia AJ, Calado ART, Ribeiro MHL. High pressure-temperature
effects on enzymatic activity: Naringin bioconversion. Food Chem 2007;102:565-570.
[122] Ferreira L, Afonso C, Vila-Real H, Alfaia A, Ribeiro MHL. Evaluation of the effect
of high pressure on naringin hydrolysis in grapefruit juice with naringinase immobilised in calcium alginate beads. Food Technol Biotech 2008;46:146-150.
[123] Ludikhuyze L, Ooms V, Weemaes C, Hendrickx M. Kinetic study of the
irreversible thermal and pressure inactivation of myrosinase from broccoli (Brassica oleracea L-Cv. Italica). J Agric Food Chem 1999;47:1794-1800.
[124] Eylen Dv, Oey I, Hendrickx M, Loey Av. Kinetics of the stability of broccoli
(Brassica oleracea cv. italica) myrosinase and isothiocyanates in broccoli juice during pressure/temperature treatments. J Agric Food Chem 2007;55:2163-2170.
[125] Mozhaev VV, Lange R, Kudryashova EV, Balny C. Application of high hydrostatic
pressure for increasing activity and stability of enzymes. Biotechnol Bioeng 1996;52:320-331.
[126] Mozhaev VV, Bec N, Balny C. Pressure effects on enzyme reactions in mainly
organic media-alpha-chymotrypsin in reversed micelles of aerosol in octane. Biochem Mol Biol Int 1994;34:191-199.
[127] Curl AL, Jansen EF. Effect of high pressures on trypsin and chymotrypsin. J Biol Chem 1950;184:45-54.
[128] Taniguchi Y, Suzuki K. Pressure inactivation of alpha-chymotrypsin. J Phys
Chem 1983;87:5185-5193. [129] Dufour E, Herve G, Haertle T. Hydrolysis of beta-lactoglobulin by thermolysin and
pepsin under high hydrostatic-pressure. Biopolymers 1995;35:475-483. [130] Morita RY, Mathemeier PF. Temperature-hydrostatic pressure studies on
partially purified inorganic pyrophosphatase activity. J Bacteriol 1964;88:1667-&. [131] Haight RD, Morita RY. Interaction between parameters of hydrostatic pressure
and temperature on aspartase of Escherichia coli. J Bacteriol 1962;83:112. [132] Ciardiello MA, Schmitt B, di Prisco G, Herve G. Influence of hydrostatic pressure
on L-glutamate dehydrogenase from the Antarctic fish Chaenocephalus aceratus. Marine Biol 1999;134:631-636.
[133] Fukushima K, Matsumoto K, Okawauchi M, Inoue T, Shimozawa R. Kinetics of
pressure-induced inactivation of bovine liver glutamate-dehydrogenase. Biochim Biophys Acta 1986;872:42-49.
[134] Saito R, Kato C, Nakayama A. Amino acid substitutions in malate
dehydrogenases of piezophilic bacteria isolated from intestinal contents of deep-sea fishes retrieved from the abyssal zone. J Gen Appl Microbiol 2006;52:9-19.
[135] Saito R, Nakayama A. Differences in malate dehydrogenases from the obligately
piezophilic deep-sea bacterium Moritella sp strain 2D2 and the psychrophilic bacterium Moritella sp strain 5710. FEMS Microbiol Lett 2004;233:165-172.
[136] Primo MS, Ceni GC, Marcon NS, Antunes OAC, Oliveira D, Oliveira JV, Dariva
C. Effects of compressed carbon dioxide treatment on the specificity of oxidase enzymatic complexes from mate tea leaves. J Supercrit Fluid 2007;43:283-290.
[137] Conesa A, Punt PJ, van den Hondel CAMJJ. Fungal peroxidases: molecular
aspects and applications. J Biotechnol 2002;93:143-158. [138] Whitaker JR, Lee CY. Recent advances in chemistry of enzymatic browning - An
overview. in: C.Y.W.J.R. Lee (Ed.), Amer Chemical Soc, 1995, pp. 2-7. [139] Asaka M, Hayashi R. Activation of polyphenoloxidase in pear fruits by high-
pressure treatment. Agric Biol Chem 1991;55:2439-2440.
[140] Asaka M, Aoyama Y, Nakanishi R, Hayashi R. Purification of a latent form of pholyphenoloixdase from la frnace pear fruit and its pressure-activation. Bioscience Biotechnology and Biochemistry 1994;58:1486-1489.
[141] Rapeanu G, Van Loey A, Smout C, Hendrickx M. Effect of pH on thermal and/or
pressure inactivation of Victoria grape (Vitis vinifera sativa) polyphenol oxidase: a kinetic study. J Food Sci 2005;70:E301-E307.
[142] Mathur EJ. Applications of thermostable DNA-polymerases in molecular biology.
ACS Sym Ser 1992;498:189-206. [143] Adams MWW, Park JB, Mukund S, Blamey J, Kelly RM. Metabolic enzymes from
sulfur-dependent, extremely thermophlic organisms. Biocatalysis at Extreme Temperatures 1992;498:4-22.
[144] Pelloux J, Rustérucci C, Mellerowicz EJ. New insights into pectin methylesterase
structure and function. Trends Plant Sci 2007;12:267-277. [145] Castro SM, Saraiva JA, Lopes-da-Silva JA, Delgadillo I, Loey AV, Smout C,
Hendrickx M. Effect of thermal blanching and of high pressure treatments on sweet green and red bell pepper fruits (Capsicum annuum L.). Food Chem 2008;107:1436-1449.
[146] Castro SM, Van Loey A, Saraiva JA, Smout C, Hendrickx M. Process stability of
Capsicum annuum pectin methylesterase in model systems, pepper puree and intact pepper tissue. Eur Food Res Technol 2005;221:452-458.
[147] Salameh Md, Wiegel J, Laskin AI, SariaslanI S, Gadd GM. Lipases from
Extremophiles and Potential for Industrial Applications. Advances in Applied Microbiology, vol. Volume 61, Academic Press, 2007, pp. 253-283.
[148] Aravindan R, Anbumathi P, Viruthagiri T. Lipase applications in food industry.
Indian Journal of Biotechnology 2007;6:141-158. [149] Gilham D, Lehner R. Techniques to measure lipase and esterase activity in vitro.
Methods 2005;36:139-147. [150] Lutz S. Engineering lipase B from Candida antarctica. Tetrahedron: Asymmetry
2004;15:2743-2748. [151] Gupta R, Gupta N, Rathi P. Bacterial lipases: an overview of production,
purification and biochemical properties. Appl Microbiol Biotechnol 2004;64:763-781.
[152] Jaeger K-E, Eggert T. Lipases for biotechnology. Curr Opin Biotechnol
2002;13:390-397.
[153] Sharma R, Chisti Y, Banerjee UC. Production, purification, characterization, and
applications of lipases. Biotechnol Adv 2001;19:627-662. [154] Beisson F, Tiss A, Riviere C, Verger R. Methods for lipase detection and assay:
a critical review. Eur J Lipid Sci Tech 2000;102:133-153. [155] Thomson CA, Delaquis PJ, Mazza G. Detection and measurement of microbial
lipase activity: A review. Crit Rev Food Sci Nutr 1999;39:165-187. [156] Yahya ARM, Anderson WA, Moo-Young M. Ester synthesis in lipase-catalyzed
reactions. Enzyme Microb Tech 1998;23:438-450. [157] Varma MN, Madras G. Kinetics of synthesis of butyl butyrate by esterification and
transesterification in supercritical carbon dioxide. J Chem Technol Biotechnol 2008;83:1135-1144.
[158] Lozano P, De Diego T, Sauer T, Vaultier M, Gmouh S, Iborra JL. On the
importance of the supporting material for activity of immobilized Candida antarctica lipase B in ionic liquid/hexane and ionic liquid/supercritical carbon dioxide biphasic media. J Supercrit Fluid 2007;40:93-100.
[159] Sabeder S, Habulin M, Knez Z. The lipase-catalyzed synthesis of fatty acid
fructose esters in organic media and in supercritical carbon dioxide. CI & CEQ 2006;12:147-151.
[160] Hernández FJ, de los Ríos AP, Gómez D, Rubio M, Víllora G. A new recirculating
enzymatic membrane reactor for ester synthesis in ionic liquid/supercritical carbon dioxide biphasic systems. Applied Catalysis B: Environmental 2006;67:121-126.
[161] Romero MD, Calvo L, Alba C, Habulin M, Primozic M, Knez Z. Enzymatic
synthesis of isoamyl acetate with immobilized Candida antarctica lipase in supercritical carbon dioxide. J Supercrit Fluid 2005;33:77-84.
[162] Matsuda T, Kanamaru R, Watanabe K, Kamitanaka T, Harada T, Nakamura K.
Control of enantioselectivity of lipase-catalyzed esterification in supercritical carbon dioxide by tuning the pressure and temperature. Tetrahedron-Asymmetry 2003;14:2087-2091.
[163] Al-Duri B, Goddard R, Bosley J. Characterisation of a novel support for
biocatalysis in supercritical carbon dioxide. J Mol Catal B: Enzym 2001;11:825-834.
[164] Rezaei K, Temelli F. Lipase-catalyzed hydrolysis of canola oil in supercritical
carbon dioxide. J Am Oil Chem Soc 2000;77:903-909.
[165] Ikushima Y, Saito N, Hatakeda K, Sato O. Promotion of a lipase-catalyzed
esterification in supercritical carbon dioxide in near-critical region. Chem Eng Sci 1996;51:2817-2822.
[166] Ikushima Y, Saito N, Arai M. Promotion of lipase-catalyzed esterification of N-
valeric acid and citronellol in supercritical carbon dioxide in the near-critical region. Journal of Chemical Engineering of Japan 1996;29:551-553.
[167] Habulin M, Knez Z. Pressure stability of lipases and their use in different
systems. Acta Chem Slove 2001;48:521-532. [168] Eisenmenger MJ, Reyes-De-Corcuera JI. High hydrostatic pressure increased
stability and activity of immobilized lipase in hexane. Enzyme Microb Tech 2009;45:118-125.
[169] Noel M, Combes D. Effects of temperature and pressure on Rhizomucor miehei
lipase stability. J Biotechnol 2003;102:23-32. [170] Osorio NM, Ribeiro MH, da Fonseca MMR, Ferreira-Dias S. Interesterification of
fat blends rich in omega-3 polyunsaturated fatty acids catalysed by immobilized Thermomyces lanuginosa lipase under high pressure. JOURNAL OF MOLECULAR CATALYSIS B-ENZYMATIC 2008;52-3:58-66.
[171] Hlavsova K, Wimmer Z, Xanthakis E, Bernasek P, Sovova H, Zarevucka M.
Lipase activity enhancement by SC-CO2 treatment. Z Naturforsch B 2008;63:779-784.
[172] Uppenberg J, Ohrner N, Norin M, Hult K, Kleywegt GJ, Patkar S, Waagen V,
Anthonsen T, Jones TA. Crystallographic and molecular-modeling studies of lipase B from Candida antarctica reveal a stereospecificity pocket for secondary alcohols. Biochemistry-US 1995;34:16838-16851.
[173] Grochulski P, Li Y, Schrag JD, Cygler M. 2 conformational states of Canadida
rudosa lipase. Protein Sci 1994;3:82-91. [174] Ericsson DJ, Kasrayan A, Johansson P, Bergfors T, Sandström AG, Bäckvall J-
E, Mowbray SL. X-ray Structure of Candida antarctica Lipase A Shows a Novel Lid Structure and a Likely Mode of Interfacial Activation. J Mol Biol 2008;376:109-119.
[175] Paraoanu LE, Layer PG. Acetylcholinesterase in cell adhesion, neurite growth
and network formation. Febs J 2008;275:618-624.
[176] Luque de Castro MD, Herrera MC. Enzyme inhibition-based biosensors and biosensing systems: questionable analytical devices. Biosens Bioelectron 2003;18:279-294.
[177] Verlent I, Hendrickx M, Verbeyst L, Van Loey A. Effect of temperature and
pressure on the combined action of purified tomato pectinmethylesterase and polygalacturonase in presence of pectin. Enzyme Microb Tech 2007;40:1141-1146.
[178] Verlent I, Smout C, Duvetter T, Hendrickx ME, Van Loey A. Effect of temperature
and pressure on the activity of purified tomato polygalacturonase in the presence of pectins with different patterns of methyl esterification. Innov Food Sci Emerg 2005;6:293-303.
[179] Verlent I, Van Loey A, Smout C, Duvetter T, Hendrickx ME. Purified tomato
polygalacturonase activity during thermal and high-pressure treatment. Biotechnol Bioeng 2004;86:63-71.
[180] van der Maarel M, van der Veen B, Uitdehaag JCM, Leemhuis H, Dijkhuizen L.
Properties and applications of starch-converting enzymes of the alpha-amylase family. J Biotechnol 2002;94:137-155.
[181] Laidler KJ. The influence of pressure on the rates of biological reactions. Arch
Biochem 1951;30:226-236. [182] Taniguchi M, Kamihira M, Kobayashi T. Effect of treatment with supercritical
carbon dioxide on enzymatic activity. Agric Biol Chem 1987;51:593-594. [183] Tanaka N, Kajimoto S, Mitani D, Kunugi S. Effects of guanidine hydrochloride
and high pressure on subsite flexibility of beta-amylase. BBA Prot Stuct M 2002;1596:318-325.
[184] Narziss L, Reicheneder E, Edney MJ. The control of beta-glucan in the brewery.
Monatsschr Brauwiss 1990;43:66-76. [185] Narziss L. Beta-glucan and beta-glucanases. Brauwissenschaft 1980;33:311-
311. [186] Tribst AAL, Franchi MA, Cristianini M. Ultra-high pressure homogenization
treatment combined with lysozyme for controlling Lactobacillus brevis contamination in model system. Innov Food Sci Emerg 2008;9:265-271.
[187] Chung W, Hancock REW. Action of lysozyme and nisin mixtures against lactic
acid bacteria. Int J Food Microbiol 2000;60:25-32.
[188] Gill AO, Holley RA. Inhibition of bacterial growth on ham and bologna by lysozyme, nisin and EDTA. Food Res Int 2000;33:83-90.
[189] Gill AO, Holley RA. Surface application of lysozyme, nisin, and EDTA to inhibit
spoilage and pathogenic bacteria on ham and bologna. J Food Prot 2000;63:1338-1346.
[190] Makki F, Durance TD. Thermal inactivation of lysozyme as influenced by pH,
sucrose and sodium chloride and inactivation and preservative effect in beer. Food Res Int 1996;29:635-645.
[191] Nattress FM, Yost CK, Baker LP. Evaluation of the ability of lysozyme and nisin
to control meat spoilage bacteria. Int J Food Microbiol 2001;70:111-119. [192] Iucci L, Patrignani F, Vallicelli M, Guerzoni ME, Lanciotti R. Effects of high
pressure homogenization on the activity of lysozyme and lactoferrin against Listeria monocytogenes. Food Control 2007;18:558-565.
[193] Orruno E, Apenten RO, Zabetakis I. The role of beta-glucosidase in the
biosynthesis of 2.5-dimethyl-4-hydroxy-3(2H)-furanone in strawberry (Fragaria x ananassa cv. Elsanta). Flavour Frag J 2001;16:81-84.
[194] Zabetakis I, Gramshaw JW, Robinson DS. 2,5-dimethyl-4-hydroxy-2H-furan-3-
one and its derivatives: analysis, synthesis and biosynthesis - a review. Food Chem 1999;65:139-151.
[195] Hamon V, Dallet S, Legoy MD. The pressure-dependence of two beta-
glucosidases with respect to their thermostability. BBA Prot Stuct M 1996;1294:195-203.
[196] Yanahira S, Suguri T, Yakabe T, Ikeuchi Y, Hanagata G, Deya E. Formation of
oligosaccharides from lactitol by aspergillus oryzae beta-D-galactosidase. Carbohydr Res 1992;232:151-159.
[197] Shin HJ, Yang JW. Galacto-oligosaccharide production by beta-galactosidase in
hydrophobic organic media. Biotechnol Lett 1994;16:1157-1162. [198] Degraeve P, Delorme P, Lemay P. Pressure-induced inactivation of E. coli [beta]-
galactosidase: influence of pH and temperatur. BBA Prot Struct M 1996;1292:61-68.
[199] Degraeve P, Lemay P. High pressure-induced modulation of the activity and
stability of Escherichia coli (lac Z) [beta]-galactosidase: Potential applications. Enzyme Microb Tech 1997;20:550-557.
[200] Goldstein H, Barry PW, Rizzuto AB, Venkatasubramanian K, Vieth WR. Continuous enzymatic production of invert sugar. Journal of Fermentation Technology 1977;55:516-524.
[201] Athes V, Combes D, Zwick A. Raman spectroscopic studies of native and
pressure- or temperature-denatured invertase. J Raman Spectrosc 1998;29:373-378.
[202] Cavaille D, Combes D. Effect of temperature and pressure on yeast invertase
stability: A kinetic and conformational study. J Biotechnol 1995;43:221-228. [203] Butz P, Ludwig H, Greulich KO. Volume changes during enzyme reactions. the
influence of pressure on the action of invertase, dextranase and dextransucrase. Biophys Chem 1978;8:163-169.
[204] Sato M, Ozawa S, Ogino Y. Effects of pressure on the sucrose inversion over an
immobilized invertase catalyst. J Phys Chem 1987;91:5755-5760. [205] Butz P, FernandezGarcia A, Lindauer R, Dieterich S, Bognar A, Tauscher B.
Influence of ultra high pressure processing on fruit and vegetable products. Elsevier Sci Ltd, 2003, pp. 233-236.
[206] Heremans L, Heremans K. Raman spectroscopic study of the changes in
secondary structure of chymotrypsin - Effect of pH and pressure on the salt bridge. Biochim Biophys Acta 1989;999:192-197.
[207] Cheret R, Hernandez-Andres A, Delbarre-Ladrat C, de Lamballerie M, Verrez-
Bagnis V. Proteins and proteolytic activity changes during refrigerated storage in sea bass (Dicentrarchus labrax L.) muscle after high-pressure treatment. European Food Research and Technology 2006;222:527-535.
[208] Kunugi S. Enzyme reactions under high pressure and their applications. Enzyme
Eng Xi 1992;672:293-304. [209] Fukuda M, Kunugi S. Pressure-dependence of thermolysin catalysis. Eur J
Biochem 1984;142:565-570. [210] Gro M, Auerbach G, Jaenicke R. The catalytic activities of monomeric enzymes
show complex pressure dependence. FEBS Lett 1993;321:256-260. [211] Kudryashova EV, Mozhaev VV, Balny C. Catalytic activity of thermolysin under
extremes of pressure and temperature: modulation by metal ions. BBA Prot Stuct M 1998;1386:199-210.
[212] Miller JF, Shah NN, Nelson CM, Ludlow JM, Clark DS. Pressure and temperature effects on growth and methane production of the extreme thermophile methanococcus jannashii. Appl Environ Microbiol 1988;54:3039-3042.
[213] Campus JFR. Inorganic pyrophosphatase Family: Pyrophosphatase, vol. 2008,
Howard Hughes Medical Institute, 2008. [214] Lahti R. Microbial inorganic pyrophosphatases. Microbiol Rev 1983;47:169-179. [215] Zancan P, Sola-Penna M. Trehalose and glycerol stabilize and renature yeast
inorganic pyrophosphatase inactivated by very high temperatures. Arch Biochem Biophys 2005;444:52-60.
[216] Viola RE. L-aspartase: New tricks from an old enzyme. Advances in Enzymology,
Vol 74, vol. 74, John Wiley & Sons Inc, New York, 2000, p. 295. [217] Asano Y, Kira I, Yokozeki K. Alteration of substrate specificity of aspartase by
directed evolution. Biomol Eng 2005;22:95-101. [218] Vanderwerf MJ, Vandentweel WJJ, Kamphuis J, Hartmans S, Debont JAM. The
potential of lyases for the industrial production of optically active compounds. Trends Biotechnol 1994;12:95-103.
[219] Welsh FW, Williams RE, Dawson KH. Lipase mediated synthesis of low-
molecular weight flavor esters. J Food Sci 1990;55:1679-1682. [220] Nemestothy N, Gubicza L, Feher E, Belafi-Bako K. Biotechnological utilisation of
fusel oil, a food industry by-product - A kinetic model on enzymatic esterification of i-amyl alcohol and oleic acid by Candida antarctica lipase B. Food Technol Biotech 2008;46:44-50.
[221] Romero MD, Calvo L, Alba C, Daneshfar A. A kinetic study of isoamyl acetate
synthesis by immobilized lipase-catalyzed acetylation in n-hexane. J Biotechnol 2007;127:269-277.
[222] Krishna SH, Manohar B, Divakar S, Prapulla SG, Karanth NG. Optimization of
isoamyl acetate production by using immobilized lipase from Mucor miehei by response surface methodology. Enzyme Microb Tech 2000;26:131-136.
[223] Rotticci D, Rotticci-Mulder JC, Denman S, Norin T, Hult K. Improved
enantioselectivity of a lipase by rational protein engineering. Chembiochem 2001;2:766-770.
[224] Lee L-s, Lin R-g. Reaction and phase equilibria of esterification of isoamyl
alcohol and acetic acid at 760 mm Hg. Fluid Phase Equilib 1999;165:261-278.
[225] Eyring H, Johnson FH, Gensler RL. Pressure and reactivity of proteins, with particular reference to invertase. J Phys Chem 1946;50:453-464.
[226] Arroyo M, Sanchez-Montero JM, Sinisterra JV. Thermal stabilization of
immobilized lipase B from Candida antarctica on different supports: Effect of water activity on enzymatic activity in organic media. Enzyme Microb Tech 1999;24:3-12.
[227] Lange R, Balny C. UV-visible derivative spectroscopy under high pressure. BBA-
Protein Struct M 2002;1595:80-93. [228] Ando N, Chenevier P, Novak M, Tate MW, Gruner SM. High hydrostatic pressure
small-angle X-ray scattering cell for protein solution studies featuring diamond windows and disposable sample cells. J Appl Chrystallogr 2008;41:167-175.
[229] Picard A, Daniel I, Montagnac G, Oger P. In situ monitoring by quantitative
Raman spectroscopy of alcoholic fermentation by Saccharomyces cerevisiae under high pressure. Extremophiles 2007;11:445-452.
[230] Tsuzuki W, Suzuki T. Reactive properties of the organic solvent-soluble lipase.
BBA-Lipid Lipid Met 1991;1083:201-206. [231] Damodaran S. Amino acids, peptides, and proteins. in: Fennema (Ed.), Food
Chemistry, Marcel Dekker Inc., New York, 1996, pp. 321-429. [232] Heremans K. High-pressure effects of proteins and other biomolecules. Annu
Rev Biophys Bioeng 1982;11:1-21. [233] Yadav GD, Devi KM. Immobilized lipase-catalysed esterification and
transesterification reactions in non-aqueous media for the synthesis of tetrahydrofurfuryl butyrate: comparison and kinetic modeling. Chem Eng Sci 2004;59:373-383.
[234] Zaidi A, Gainer JL, Carta G, Mrani A, Kadiri T, Belarbi Y, Mir A. Esterification of
fatty acids using nylon-immobilized lipase in n-hexane: kinetic parameters and chain-length effects. J Biotechnol 2002;93:209-216.
[235] Balny C, Mozhaev VV, Lange R. Hydrostatic pressure and proteins: Basic
concepts and new data. Comparative Biochemistry and Physiology a-Physiology 1997;116:299-304.
[236] Katsaros GI, Katapodis P, Taoukis PS. Modeling the effect of temperature and
high hydrostatic pressure on the proteolytic activity of kiwi fruit juice. J Food Eng 2009;94:40-45.
[237] Van Rantwijk F, Sheldon RA. Biocatalysis in ionic liquids. Chem Rev 2007;107:2757-2785.
[238] Dang DT, Ha SH, Lee S-M, Chang W-J, Koo Y-M. Enhanced activity and stability
of ionic liquid-pretreated lipase. J Mol Catal B: Enzym 2007;45:118-121. [239] Nara SJ, Harjani JR, Salunkhe MM. Lipase-catalysed transesterification in ionic
liquids and organic solvents: a comparative study. Tetrahedron Lett 2002;43:2979-2982.
[240] Lou WY, Zong MH, Liu YY, Wang JF. Efficient enantioselective hydrolysis of d,l-
phenylglycine methyl ester catalyzed by immobilized Candida antarctica lipase B in ionic liquid containing systems. J Biotechnol 2006;125:64-74.
[241] Noel M, Lozano P, Vaultier M, Iborra JL. Kinetic resolution of rac-2-pentanol
catalyzed by Candida antarctica lipase B in the ionic liquid, 1-butyl-3-methylimidazolium bis[(trifluoromethyl)sulfonyl]amide. Biotechnol Lett 2004;26:301-306.
[242] Feher E, Major B, Belafi-Bako K, Gubicza L. Semi-continuous enzymatic
production and membrane assisted separation of isoamyl acetate in alcohol-ionic liquid biphasic system. Desalination 2009;241:8-13.
[243] Cao L, Langen Lv, Sheldon RA. Immobilised enzymes: carrier-bound or carrier-
free? Curr Opin Biotechnol 2003;14:387-394. [244] Lozano P, Perez-Marin AB, De Diego T, Gomez D, Paolucci-Jeanjean D,
Belleville MP, Rios GM, Iborra JL. Active membranes coated with immobilized Candida antarctica lipase B: preparation and application for continuous butyl butyrate synthesis in organic media. Journal of Membrane Science 2002;201:55-64.
[245] Lozano P, De Diego T, Carrie D, Vaultier M, Iborra JL. Enzymatic catalysis in
ionic liquids and supercritical carbon dioxide. in: R.D. Rodgers, K.R. Seddon (Eds.), 2003, pp. 239-250.
[246] Lozano P, De Diego T, Carrie D, Vaultier M, Iborra JL. Enzymatic ester synthesis
in ionic liquids. J Mol Catal B: Enzym 2003;9-13. [247] Zhao H, Baker GA, Song ZY, Olubajo O, Zanders L, Campbell SM. Effect of ionic
liquid properties on lipase stabilization under microwave irradiation. Journal of Molecular Catalysis B-Enzymatic 2009;57:149-157.
[248] Rios A, Hernandez-Fernandez FJ, Tomas-Alonso F, Gomez D, Villora G.
Synthesis of flavour esters using free Candida antarctica lipase B in ionic liquids. Flavour Frag J 2008;23:319-322.
[249] Goossens K, Smeller L, Heremans K. Pressure tuning spectroscopy of the low
freqency raman-spectrum of liquid amides. J Chem Phys 1993;99:5736-5741. [250] Dzwolak W, Kato M, Taniguchi Y. Fourier transform infrared spectroscopy in
high-pressure studies on proteins. BBA Prot Struct M 2002;1595:131-144. [251] Kremer W. High-pressure NMR studies in proteins. Annual Reports on Nmr
Spectroscopy, Vol 57, vol. 57, Elsevier Academic Press Inc, San Diego, 2006, pp. 177-203.
[252] Lange R, Frank J, Saldana JL, Balny C. Fourth derivative UV-spectroscopy of
proteins under high pressure .1. Factors affecting the fourth derivative spectrum of the aromatic amino acids. European Biophysics Journal with Biophysics Letters 1996;24:277-283.
[253] Lange R, Bec N, Mozhaev VV, Frank J. Fourth derivative UV-spectroscopy of
proteins under high pressure .2. Application to reversible structural changes. European Biophysics Journal with Biophysics Letters 1996;24:284-292.
[254] Ruan K, Balny C. High pressure static fluorescence to study macromolecular
structure-function. BBA Prot Struct M 2002;1595:94-102. [255] Cioni P, Strambini GB. Tryptophan phosphorescence and pressure effects on
protein structure. BBA Prot Struct M 2002;1595:116-130.
BIOGRAPHICAL SKETCH
Michael was born and raised in Grand Island Nebraska. After high-school he
completed his B.S. in animal science and his M.S. in food science at Oklahoma State
University in Stillwater Oklahoma. After working as a research specialist he began his
Ph.D. in food science at the University of Florida. Michael has served as the IFT-Florida
section executive student representative, as the captain of the UF college bowl team, as
captain of the Dansico product development team, as a member of the UF IFTSA
product development team, and is active in a variety of other extracurricular activities.
Michael’s research Interests include improving the application and understanding
of enzyme catalysis through use of novel and innovative technologies with focus on
utilization of high pressure. His research has recently gained much attention after being
awarded 1st place in the biotechnology division poster competition at the 2008 IFT
annual meeting & Expo and 3rd place at the 2009 International Commission of
Agricultural and Biosystems Engineering International Technical Symposium in
Potsdam Germany. Michael research has been, and will continue to be published and
cited in renowned scholarly journals and discussed at technical conferences.
Upon completion of the requirements for a Ph.D. in food science at the University
of Florida Michael intends to seek a position within the food industry to apply his current
and developing skill set to improve the availability and nutritional quality of the world’s
food supply.