Post on 17-Jan-2018
description
Genome mining and annotation validation
Georges Cohen
Institut Pasteur Paris
e-mail:gncohen@pasteur.fr
As many as 40% of all predicted genes in completed prokaryotic genomes have no functional annotation
Many genes have a predicted function, but that prediction has not been experimentally validated
As many as 5-10% of predicted gene functions may be incorrect
Many known enzymes have no corresponding genes identified in the
sequence databases
- Known since the 50’s-1 mole of lysine is degraded to 1 mole of acetate,1 mole of butyrate and 2 moles NH3Well studied in Clostridium sticklandii, but also present in Porphyromonas gingivalis and Fusobacterium nucleatum
Lysine fermentation
Lysine fermentation in Fusobacterium nucleatum Lysine 2,3-
aminomutase
C O O H
ON H2
N H3
Notsequenced
-Lysine 5,6-aminomutase
A c e t y l - C o A
S C o A
ON H2
O H
OO
Not sequenced
S C o A
O
S C o A
O
N H3
Not sequenced
Acyl-CoAdehydrogenase
O H
O
S C o A
OO
Butyrate-CoAacetoacetyl-CoA
transférase
A c e t y l - C o A A c e t a t e
C o A S H
A T P
A D P + P i
C o A S H
Acetyl-CoAacetyltransférase
COOH
NH2
H2N
COOHH2N
NH2
COOH
NH2NH2
Lysine kamAkamD,E
AtoA,D
C O O H
N H2
N H2
C O O H
ON H2
Data mining for the 3,5-diaminohexanoate dehydrogenase encoding gene
NH3
Characteristics of 3,5-diaminohexanoate dehydrogenase: -isolated and purified from Clostridium SB4, Clostridium sticklandii, Brevibacterium L5- cofactor: NAD+- molecular weight between 37 and 39 kDa- dimer or tetramer
Search for a F.nucleatum protein which a) possesses a binding site for NAD+ b) has a molecular weight around 38 kDa
H2O
+ NADH + H+NAD +
Best candidate: FN1867
Substrate L-erythro-3,5-diaminohexanoate
C O O H
N H2
N H2
**2 stereoisomeric centers 4 stereoisomers
C H2
C H
C H2
H C
C H3
C O O H
H2
N
N H2
C H2
H C
C H2
H C
C H3
N H2
N H2
C O O H
C H2
H C
C H2
C H
C H3
N H2
C O O H
H2
N
C H2
C H
C H2
C H
C H3
C O O H
H2
N
H2
N
L-erythro D-erythro L-threo D-threo
C O O H
N
H
O
N H2
C O O H
N H2
N H2
Synthesis of DL-erythro-3,5-diaminohexanoate
Références: Chem. Berichte 1904, 37, 2357-2362 Organic Preparations and Procedures Int. 1973, 5, 31-35
+ NH3
150 °C, 20 hUnder pressure
+ HCl
6 hrefluxSorbic acid DL-erythro-
3,5-diaminohexanoate- Separation of erythro and threo by recrystallisation in isopropanol- no separation of the D et L isomers
Lysine fermentation in Fusobacterium nucleatum
Lysine 2,3-aminomutase
C O O H
ON H2
N H3
Notsequenced
-Lysine 5,6-aminomutase
A c e t y l - C o A
S C o A
ON H2
O H
OO
Not sequenced
S C o A
O
S C o A
O
N H3
Not sequenced
Acyl-CoAdehydrogenase
O H
O
S C o A
OO
Butyrate-CoAacetoacetyl-CoA
transférase
A c e t y l - C o A A c e t a t e
C o A S H
A T P
A D P + P i
C o A S H
Acetyl-CoAacetyltransférase
COOH
NH2
H2N
COOHH2N
NH2
COOH
NH2NH2
Lysine kamAkamD,E
AtoA,D
Enzymatic assay for FN 1868
COOH
NH2NH2
COOH
ONH2+ NAD NH4
++ + H2O + +NADH H+
1) Let the product of FN1867 accumulate
FN1867
L-erythro-3,5-DAH 3-Keto-5-aminohexanoate
SCoA
ONH2
OH
OO
COOH
ONH2+ acetyl-CoA +
FN1868
2) Add then FN1868 and the co-substrate acetyl CoA
3-Keto-5-aminohexanoate 3-aminobutyryl-CoA
3) Follow the disappearance of’acetyl CoA using citrate synthase(CS)
acetyl-CoA + oxaloacetate+ DTNB citrate + CoA-disulfite + thionitrobenzoateCS
absorbance at 412 nm
Tri-coupled assay for FN1869
Diaminohexanoate------> 3-keto-5-aminohexanoate----->3-aminobutyryl CoA
----> Crotonyl CoA
FN1867 FN1868
-----
FN1869
Annett KreimeyerAlain PerretClaudine MédigueMarcel SalanoubatJean WeissenbachJ.Biol.Chem.,(2007)282,7191-7
Georges Cohen, consultant