Molecular BiologyFourth Edition
Chapter 17
The Mechanism of Translation I: Initiation
Robert F. Weaver
Chapter 18The Mechanism of Translation II: Elongation and Termination
Chapter 19
Ribosomes and Transfer RNA
17-2
17.1 Initiation of Translation in Bacteria
• Two important events must occur before translation initiation can take place– Generate a supply of aminoacyl-tRNAs
• Amino acids must be covalently bound to tRNAs• Process of bonding tRNA to amino acid is called
tRNA charging
– Dissociation of ribosomes into their two subunits
• The cell assembles the initiation complex on the small ribosomal subunit
• The two subunits must separate to make assembly possible
17-3
tRNA Charging• All tRNAs have same 3
bases at 3’-end (CCA)• Terminal adenosine is
the target for charging with amino acid
• Amino acid attached by ester bond between – Its carboxyl group – 2’- or 3’-hydroxyl group
of terminal adenosine of tRNA
Amino acid
17-4
Two-Step Charging
• Aminoacyl-tRNA synthetases join amino acids to their cognate tRNAs
• This is done in a two-step reaction:– Begins with activation of the amino acid with
AMP derived from ATP– In the second step, the energy from the
aminoacyl-AMP is used to transfer the amino acid to the tRNA
17-5
Aminoacyl-tRNA Synthetase Activity
AMP/amino acid coupling
AMP/tRNA displacement
17-6
Dissociation of Ribosomes• E. coli ribosomes
dissociate into subunits at the end of each round of translation
• IF1 actively promotes this dissociation
• IF3 binds to free 30S subunit and prevents reassociation with 50S subunit to form a whole ribosome
17-7
Ribosomal Subunit Exchange
Grow in heavy isotope of nitrogen, carbon, and hydrogen. Then 3H labeled
17-8
Formation of the 30S Initiation Complex
When ribosomes have been dissociated into 50S and 30S subunits, cell builds a complex on the 30S subunit:
– mRNA– Aminoacyl-tRNA– Initiation factors
• IF3 binds by itself to 30S subunit• IF1 and IF2 stabilize this binding• IF2 can bind alone, but is stabilized with help of
IF1 and IF3• IF1 does not bind alone
17-9
First Codon and the First Aminoacyl-tRNA
• Prokaryotic initiation codon is:– Usually AUG– Can be GUG– Rarely UUG
• Initiating aminoacyl-tRNA is N-formyl-methionyl-tRNA
• N-formyl-methionine (fMet) is the first amino acid incorporated into a polypeptide
• This amino acid is frequently removed from the protein during maturation
17-10
N-Formyl-Methionine
Lipman et al.,
Marcker and Sanger
17-11
Formyl-Met-tRNA and Met-tRNA
• Which codons they respond to?
• Which position within the protein they placed methionine?
17-12
Which codons they respond to?
• Make a labeled aminoacyl-tRNA, mix it with ribosomes and a variety of trinucleotides, such as AUG.
• Met-tRNA bind AUG, formyl-Met-tRNA binds AUG, GUG, and UUG.
AUG >90% , GUG about 8% UUG 1%
17-13
Which position within the protein they placed methionine?
• mRNA Sequence AUG AUG AUG…….• In vitro translation system
– In the presence of tRNAmet, met is incorporated into interior of the product
– In the presence of formy-tRNAmet, met is incorporated into the first codon of the product
Weigert and Garen:Formyl-Met of the the polypeptide is always removed in bacteria and phage proteins
17-15
Binding mRNA to the 30S Ribosomal Subunit
• The 30S initiation complex is formed from a free 30S ribosomal subunit plus mRNA and fMet-tRNA
• Binding between the 30S prokaryotic ribosomal subunit and the initiation site of a message depends on base pairing between– Short RNA sequence
• Shine-Dalgarno sequence• Upstream of initiation codon
– Complementary sequence• 3’-end of 16S RNA
Binding mRNA and fMet-tRNA to the 30S ribosomal subunit
How does the cell detect the difference between the initiation codon and an
ordinary codon with the same sequences?
Consensus sequences?Consensus sequences?
17-17
Positive strand phages
• R17
• f2
• MS2– Positive strand phages– Encode three genes: A (maturation) protein,
coat protein and replicase
17-18
Gene structure of MS2 phage RNA
17-19
The secondary structures have inhibitory effect
17-20
• Lodish et al:– Translating f2 coat mRNA by ribosomes from
different bacteria– B. stearothermophilus could only translate A
protein but not coat protein– (This is not due to initiation factors but
ribosomes)
17-21
• Nomura et al.,• The important element is in the 30S
ribosome– If the 30S ribosome from the E. coli, the coat
protein can be translated– If the 30S ribosome from the B.
stearothermophilus, the coat protein can not be translated
• The active elements are S12 and 16S rRNA
17-22
• Shine and Dalgarno• Upstream of initiation codon: 5’- AGGAGGU
• 3’ end of the 16S rRNA: 3’HO-AUUCCUCCAC
• B. stearothermophilus has poor match
17-23
• Bacillus 16S rRNA– 4 Watson Crick base pairing with the A protein
and replicase ribosome binding sites– 2 with the coat protein gene
• E. coli– At least three base pairs with all three genes
Could the base pairing between 16S rRNA and the region upstream of the translation initiation site be vital to ribosome binding?
Shine-Dalgarno (SD) sequence
See Table 17.1
AGGAGGU
From ribosomes from C. crescentus and P. aeruginosa
No ribosome binding would occur for less than 3 bp
17-25
17-26
• Steitz and Jakes
• Ribosome from E. coli bound to initiation site and treated with Colicin E3 (RNase)
• Fingerprinting– Initiation site including S-D sequence– An oligonucleotide from 3’end of the 16S
rRNA
17-27
The best evidence• Hui and De Boer in 1987• Clone the human growth hormone gene
into E. coli
TranslationWT SD sequence
WT 16S rRNA
GGAGG
CCUCC (5 pairing)
OK
SD sequence
16S rRNA
CCUCC
CCUCC (no pairing)
NO
SD sequence
16S rRNA
GUGUG
CCUCC (2 pairing)
NO
SD sequence
16S rRNA
CCUCC
GGAGG (5 pairing)
OK
17-28
Initiation Factors and 30S Subunit
• Binding of the Shine-Dalgarno sequence with the complementary sequence of the 16S rRNA is mediated by IF3– Assisted by IF1 and IF2– All 3 initiation factors have bound to the
30S subunit at this time
17-29
Binding of fMet-tRNA to the 30S Initiation Complex
• IF2 is the major factor promoting binding of fMet-tRNA to the 30S initiation complex
• Two other initiation factors also play an important supporting role
• GTP is also required for IF2 binding at physiological IF2 concentrations
• The GTP is not hydrolyzed in the process
17-30
30S Initiation Complex
The complete 30S initiation complex contains one each:
– 30S ribosomal subunit– mRNA– fMet-tRNA– GTP– Factors IF1, IF2, IF3
17-31
Formation of the 70S Initiation Complex
• GTP is hydrolyzed after the 50S subunit joins the 30S complex to form the 70S initiation complex
• This GTP hydrolysis is carried out by IF2 in conjunction with the 50S ribosomal subunit
• Hydrolysis purpose is to release IF2 and GTP from the complex so polypeptide chain elongation can begin
What is the function of GTP hydrolysis
GTP hydrolysis is to remove IF-2 from the ribosomes
Exp: 30S initiation complex+labeled IF-2 and fMet-tRNA and either GDPCP or GTP, add 50S and ultracentrifugation
17-33
17.18 Effect of GTP hydrolysis on release of IF-2 from the ribosome.
After adding 50S, IF-2 is released from the 70S ribosome but fmet-tRNA is still associated
17-34
• In Fig 17.18, more fMet-tRNA is associated with the 70S ribosomes
• Catalytic function of IF2
– Hydrolysis of GTP is necessary to release IF2 from the 70S initiation complex so it can bind another molecule of fmet-tRNA, otherwise, IF2 only acts stoichiometrically
17-35
Bacterial Translation Initiation1. IF1 influences dissociation of
70S ribosome to 50S and 30S
2. Binding IF3 to 30S, prevents subunit reassociation
3. IF1, IF2, GTP bind alongside IF3
4. Binding mRNA to fMet-tRNA forming 30S initiation complexa. Can bind in either orderb. IF2 sponsors fMet-tRNAc. IF3 sponsors mRNA
5. Binding of 50S with loss of IF1 and IF3
6. IF2 dissociation and GTP hydrolysis
17-36
17.2 Initiation in Eukaryotes•Eukaryotic
– Begins with methionine– Initiating tRNA not same
as tRNA for interior – No Shine-Dalgarno– mRNA have caps at
5’end
• Bacterial– N-formyl-methionine– Shine-Dalgarno
sequence to show ribosomes where to start
17-37
Scanning Model of Initiation• Eukaryotic 40S ribosomal subunits locate
start codon by binding to 5’-cap and scanning downstream to find the 1st AUG in a favorable context
• Kozak’s Rules are a set of requirements• Best context uses A of ACCAUGG as +1:
– Purine (A or G) in -3 position– G in +4 position
• 5-10% cases ribosomal subunits bypass 1st AUG scanning for more favorable one
The scanning model of initiationKozak systematically mutated nucleotides around the initiation ↓codon in a cloned rat preproinsulin gene ↓Introduce into COS cells↓
Label newly synthesized protein with 35S-Met↓
Immunoprecipitate ↓Electrophoresis↓Detect by autoradipgraph
The scanning model of initiation
The better the translation initiation, the more proinsulin was made
17-40
The best initiation occur with a G or an A in position –3 and a G in position +4 (where the A in ATG is position +1)
A/G C C A T G G -3 -2 -1 +1 +2 +3 +4
17-41
Figure 17.21 Effects of single base changes in positions –3 and +4 surrounding the initiating ATG.
17-42
If this really is the optimum sequence for translation initiation, introducing it out of frame and upstream of the normal initiation codon should provide a barrier to scanning ribosomes and force them to initiate out of frame
17-43
The closer it resembled the optimal sequence, the more it interfered with initiation at the downstream ATG
Out-of-frame ATG
17-44
Translation With a Short ORF
• Ribosomes can use a short upstream open reading frame: – Initiate at an upstream AUG– Translate a short Open Reading Frame– Continue scanning– Reinitiate at a downstream AUG
17-45
Scanning Model for Translation Initiation
17-46
Effects of mRNA Secondary Structure
• Secondary structure near the 5’-end of an mRNA can have either positive or negative effects
• Hairpin just past an AUG can force a pause by ribosomal subunit and stimulate translation
• Very stable stem loop between cap and initiation site can block scanning and inhibit translation
17-47
Eukaryotic Initiation Factors
• Bacterial translation initiation requires initiation factors as does eukaryotic initiation of translation
• Eukaryotic system is more complex than bacterial– Scanning process– Factors to recognize the 5’-end cap
17-48
Translation Initiation in EukaryotesEukaryotic initiation factors and general functions:• eIF2 binds Met-tRNA to ribosomes• eIF2B activates eIF2 replacing its GDP with GTP• eIF1 and eIF1A aid in scanning to initiation codon• eIF3 binds to 40S ribosomal subunit, inhibits reassociation
with 60S subunit• eIF4 is a cap-binding protein allowing 40S subunit to bind 5’-
end of mRNA• eIF5 encourages association between 60S ribosome subunit
and 48S complex• eIF6 binds to 60S subunit, blocks reassociation with 40S
subunit
Fig. 17.22
17-49
Function of eIF4
• eIF4 is a cap-binding protein
• This protein is composed of 3 parts:– eIF4E, 24-kD, has actual cap binding activity– eIF4A, a 50-kD polypeptide– eIF4G is a 220-kD polypeptide
• The complex of the three polypeptides together is called eIF4F
17-50
The cap-binding proteins
GDP-binding protein
Cap binding protein
17-51
Function of eIF4A and eIF4B
• eIF4A – Has an RNA helicase activity– This activity unwinds hairpins found in the 5’-
leaders of eukaryotic mRNA– Unwinding activity is ATP dependent
• eIF4B – Has an RNA-binding domain– Can stimulate the binding of eIF4A to mRNA
17-52
Function of eIF4G
• eIF4G is an adaptor protein capable of binding to other proteins including:– eIF4E, cap-binding protein– eIF3, 40S ribosomal subunit-binding protein– Pab1p, a poly[A]-binding protein
• Interacting with these proteins lets eIF4G recruit 40S ribosomal subunits to mRNA and stimulate translation
17-53
Fig. 17.27
Inhibit capped cellular mRNA
Synergy effect
1. Regulatory protein and miRNA bound to the 3’UTR are close to the cap, which could help them influence the cap
2. Ribosomes copleteing one round of translation are close to the cap
3. Unavailable to RNase
17-54
Structure and Function of eIF3• eIF3 is a 5-lobed protein that binds at the same
site to: – eIF4G– Prominent part of viral IRES
• This explains how the IRES can substitute for 40S ribosomal subunit to mRNA
• Cryo-EM studies have produced a model for the eIF3-IRES-40S complex explaining how eIF3 prevents premature 40S-60S association (sits at the site of proposed key contact between two particles)
17-55
Prevention of Premature 40S-60S Association
• eIF3 blocks key contact point between subunits 40S and 60S
• eIF4G, so also eIF4E, locate close to the cap on an mRNA bound to 40S ribosomal particle
• eIF4 would be in position to cap-bind
17-56
Functions of eIF1 and eIF1A• eIF1 and eIF1A act synergistically to promote
formation of a stable 48S complex involving:– Initiation factors
– Met-tRNA
– 40S ribosomal subunits bound at initiation codon of mRNA
• eIF1 and eIF1A act by – Dissociating improper complexes between 40S
subunits and mRNA
– Encouraging formation of stable 48S complexes
17-57
Principle of the Toeprint Assay
Source: Adapted from Jackson, R., J. G. Sliciano, Cinderella factors have a ball, Nature 394:830, 1998.
17-58
Preformed complex I is not a dead end
Marker17.32
17-59
Functions of eIF5 and eIF5B (eIF5 encourages association between 60S ribosome subunit
and 48S complex)• eIF5B is homologous to prokaryotic factor IF2
– Binds GTP• Uses GTP hydrolysis to promote its own
dissociation from ribosome• Permits protein synthesis to begin
– Stimulates association of 2 ribosomal subunits
• Differs from IF2 as eIF5B cannot stimulate binding of initiating aminoacyl-tRNA to small ribosomal subunit
• eIF5B works with eIF5
17-60
17.3 Control of Initiation• Given the amount of control at the
transcriptional and posttranscriptional levels, why control gene expression at translational level?
• Major advantage = speed– New gene products can be produced quickly – Simply turn on translation of preexisting
mRNA• Valuable in eukaryotes• Transcripts are relatively long• Take correspondingly long time to make
– Most control of translation happens at the initiation step
17-61
Bacterial Translational Control• Most bacterial gene expression is
controlled at transcription level• Majority of bacterial mRNA has a very
short lifetime– Only 1 to 3 minutes– Allows bacteria to respond quickly to
changing circumstances
• Different cistrons on a polycistronic transcript can be translated better than others
17-62
Shifts in mRNA Secondary Structure
• mRNA secondary structure can govern translation initiation– Replicase gene of the MS2 class of phages
• Initiation codon is buried in secondary structure until ribosomes translating the coat gene open up the structure
– Heat shock sigma factor,32 of E. coli• Repressed by secondary structure that is relaxed
by heating• Heat can cause an immediate unmasking of
initiation codons and burst of synthesis
17-63
Proteins/mRNAs Induce mRNA Secondary Structure Shifts
• Small RNAs with proteins can affect mRNA 2° structure to control translation initiation
• Riboswitches can be used to control translation initiation via mRNA 2° structure– 5’-untranslated region of E. coli thiM mRNA
contain a riboswitch– This includes an aptamer that binds thiamine
and its metabolite• Thiamine phosphate• Thiamine pyrophosphate (TTP)
17-64
Activation of mRNA Translation• When TPP abundant
– Binds aptamer– Causes conformational shift
in mRNA– Ties up Shine-Dalgarno in
2° structure• Shift hides the SD sequence
from ribosomes– Inhibits translation of mRNA
• Saves energy as thiM mRNA encodes an enzyme needed to produce more thiamine and TPP
17-65
Eukaryotic Translational Control• Eukaryotic mRNA lifetimes are relatively long, so
there is more opportunity for translation control than in bacteria
• eIF2 -subunit is a favorite target for translation control– Heme-starved reticulocytes activate HCR (heme-
controlled repressor) • Phosphorylates eIF2• Inhibit initiation
– Virus-infected cells have another kinase, DAI– Phosphorylates eIF2– Inhibits translation initiation
17-66
Repression of Translation by Phosphorylation
17-67
Phosphorylation of an eIF4E-Binding Protein
• Insulin and a number of growth factors stimulate a pathway involving a protein kinase known as mTOR
• mTOR kinase’s target protein– PHAS-1 (rat)– 4E-BP1 (human)
• Once phosphorylated by mTOR– This protein dissociates from eIF4E– Releases it to participate in active translation
initiation
17-68
Stimulation of Translation by Phosphorylation of PHAS-1
17-69
Blockage of Translation Initiation by an miRNA
• miRNA controls gene expression in two ways:– Degradation of mRNA when base-paired perfectly– Inhibition of protein production if not perfect match
• Filipowicz et al conTranslation initiation that is cap-independent due to presence of an IRES, or a tethered initiation factor, is not affected by let-7 miRNA– This miRNA blocks binding of eIF4E to the cap of
target mRNAs in the human cell
17-70
RNA Degradation
80%
20%
P1573-
10x 10x
17-71
Blockage of Translation Initiation by an miRNA
• The let-7 miRNA shifts the polysomal profile of target mRNAs in human cells toward smaller polysomes– This miRNA blocks translation initiation in human cells
• Translation initiation that is cap-independent due to presence of an IRES, or a tethered initiation factor, is not affected by let-7 miRNA– This miRNA blocks binding of eIF4E to the cap of
target mRNAs in the human cell
17-72
Fig. 17.46
Polysomes: A mRNA attached to several ribosomes (Ch. 19)
Anti-miRNA inhibitor revert this effect
The more active translation initiation, the more ribosome will attach to the mRNA
Collect and fractionate polysomes from cells transfected with RL-3xBulge gene and perform Northern blotting
17-73
Fig. 17.47
17-74
Blockage of Translation Initiation by an miRNA
• Lin-4 miRNA does not alter the polysome profile of its target mRNA in C. elegans and does not appear to block translation initiation. – Different miRNAs have different modes-of-
action– miRNAs work differently in different organisms– Or both
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