and initiation codons in mycoplasmas optimizes initiation...
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RNA Biology
ISSN: 1547-6286 (Print) 1555-8584 (Online) Journal homepage: http://www.tandfonline.com/loi/krnb20
Coevolution of the translational machineryoptimizes initiation with unusual initiator tRNAsand initiation codons in mycoplasmas
Shreya Ahana Ayyub, Divya Dobriyal, Riyaz Ahmad Shah, Kuldeep Lahry,Madhumita Bhattacharyya, Souvik Bhattacharyya, Saikat Chakrabarti &Umesh Varshney
To cite this article: Shreya Ahana Ayyub, Divya Dobriyal, Riyaz Ahmad Shah, Kuldeep Lahry,Madhumita Bhattacharyya, Souvik Bhattacharyya, Saikat Chakrabarti & Umesh Varshney (2017):Coevolution of the translational machinery optimizes initiation with unusual initiator tRNAs andinitiation codons in mycoplasmas, RNA Biology, DOI: 10.1080/15476286.2017.1377879
To link to this article: http://dx.doi.org/10.1080/15476286.2017.1377879
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Coevolution of the translational machinery optimizes initiation with unusual initiator tRNAs and
initiation codons in mycoplasmas
Shreya Ahana Ayyub1, Divya Dobriyal
1, Riyaz Ahmad Shah
1, Kuldeep Lahry
1,Madhumita Bhattacharyya
2,
Souvik Bhattacharyya1, Saikat Chakrabarti
2 and Umesh Varshney
1,3,*
1Department of Microbiology and Cell Biology, Indian Institute of Science, Bangalore 560012, India
2CSIR-Indian Institute of Chemical Biology, Kolkata 700032
3Jawaharlal Nehru Centre for Advanced Scientific Research, Jakkur, Bangalore, 560064
*Correspondence to: Umesh Varshney, Phone: +918022932686, Fax: +918023602697, E-mail:
[email protected]; [email protected]
Abstract
Initiator tRNAs (i-tRNAs) are characterized by the presence of three consecutive GC base pairs (GC/GC/GC)
in their anticodon stems in all domains of life. However, many mycoplasmas possess unconventional i-tRNAs
wherein the highly conserved sequence of GC/GC/GC is represented by AU/GC/GC, GC/GC/GU or
AU/GC/GU. These mycoplasmas also tend to preferentially utilize non-AUG initiation codons. To investigate
if initiation with the unconventional i-tRNAs and non-AUG codons in mycoplasmas correlated with the
changes in the other components of the translation machinery, we carried out multiple sequence alignments of
genes encoding initiation factors (IF), 16S rRNAs, and the ribosomal proteins such as uS9, uS12 and uS13. In
addition, the occurrence of Shine-Dalgarno sequences in mRNAs was analyzed. We observed that in the
mycoplasmas harboring AU/GC/GU i-tRNAs, a highly conserved position of R131 in IF3, is represented by
P, F or Y and, the conserved C-terminal tail (SKR) of uS9 is represented by the TKR sequence. Using the
Escherichia coli model, we show that the change of R131 in IF3 optimizes initiation with the AU/GC/GU i-
tRNAs. Also, the SKR to TKR change in uS9 was compatible with the R131P variation in IF3 for initiation
with the AU/GC/GU i-tRNA variant. Interestingly, the mycoplasmas harboring AU/GC/GU i-tRNAs are also
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human pathogens. We propose that these mycoplasmas might have evolved a relaxed translational apparatus
to adapt to the environment they encounter in the host.
Keywords
mycoplasma, initiator tRNA, IF3, ribosome, evolution
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Introduction
The eubacterial initiator tRNAfMet
(i-tRNA) plays an important role in selecting the start codon. Two
of the most crucial features of the bacterial i-tRNA important in its targeting to the ribosomal P-site are the
formylation of the amino acid attached to it, and the presence of 3 consecutive GC base pairs (GC/GC/GC) in
its anticodon stem1-3
. Of these, the presence of the three GC base pairs is highly conserved in all domains of
life. Interestingly, one of the many singular distinctive features of mycoplasma, and the α-proteobacteria (like
the Rhizobium species) across the different species is the frequent presence of variations in the anticodon stem
sequences of i-tRNAs (Fig. 1). While the i-tRNAs in many α-proteobacteria possess a variant AU pair in
place of the 1st GC pair (AU/GC/GC), many mycoplasmal species have i-tRNAs with variations at the 1
st
and/or the 3rd
GC base pairs (AU/GC/GC, AU/GC/GU, or GC/GC/GU).
Selection of tRNAfMet
at the P-site is orchestrated by the P-site elements of the ribosome and the
initiation factors4-8
(Fig. 2). The P-site elements include the 16S rRNA residues (G1338 and A1339)9, 10
, the
m2G966 and m
5C967 methylations (carried out by RsmD and RsmB, respectively)
11, and the C-terminal tails
of 30S ribosomal protein uS9 and uS136, 11, 12
. The nature of Shine-Dalgarno (SD) and anti-SD (aSD)
interactions13
and the rate of 50S association with the 30S pre-initiation complex also contribute to the
selection of i-tRNA on ribosome8, 14
. Studies in Escherichia coli from our lab stemming from the naturally
occurring changes in the 3GC pairs revealed that only the 2nd
GC pair is essential for i-tRNA function15
and
subsequent investigations revealed that it is specifically the ‘G’ of the 2nd
GC pair (G30) which is the most
crucial nucleotide16
. Although an AU/GC/GU anticodon stem mutant i-tRNA can sustain E. coli, it
substantially impairs the growth and overall fitness of the cell15
. The 3GC base pairs license i-tRNA
transitions from the 30S initiation complex to the 70S initiation complex and then to an elongation competent
70S complex following the release of IF316
. More recent work from our laboratory has also shown that the
presence of intact 3GC base pairs is crucial for ribosome maturation3. As many mycoplasmal species are
sustained on AU/GC/GU i-tRNA, it is reasonable to postulate that they may have coevolved with other
genetic variations for an optimal utilization/P-site accommodation of the AU/GC/GU i-tRNA. For instance, it
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has been reported that mycoplasmal species lack various methyltransferases required for methylations of 16S
rRNA residues17
. Homologs of RsmB and RsmF (which methylate 16S rRNA at positions 967 and 1407) are
present in Mycoplasma species which are sustained on the conserved GC/GC/GC i-tRNAs (M. capricolum,
M. mycoides and M. synoviae) but not in the species lacking even one pair of the conserved 3GC base pairs.
RsmA, which methylates positions 1518 and 1519 in 16S rRNA is conserved across all the species studied.
Observations regarding the presence of RsmC and RsmD were inconclusive, as they were not distributed in
any clear pattern. Mutations in methyltransferases (RsmB, RsmD and RsmF) in E. coli led to an elevated
initiation with a mutant i-tRNA (3GC mutant) wherein the GC/GC/GC base pairs were changed to those
found in the elongator species of tRNAMet
(UA/CG/AU), indicating a likely evolutionary association between
16S rRNA methylation and the i-tRNA anticodon stem sequence.
This led us to wonder whether the organisms utilizing the variant i-tRNAs possess any other unique
features in their translational apparatus to facilitate accommodation of the unconventional i-tRNA in the
ribosomal P-site, for mRNA translation. To carry out a systematic analysis to address this question, we chose
to investigate the features of the translational apparatus in mycoplasma. An advantage the mycoplasmas offer
for such analyses is that they represent minimal genome sizes and that within the same genus, there exist
different species which use i-tRNAs possessing either the conventional GC/GC/GC sequence or its
unconventional variants. We carried out a computational analysis of the protein/RNA sequences. Among the
various translation factors, IF3 (encoded by infC gene) plays a crucial role in i-tRNA selection and is known
to inspect the i-tRNA for the 3GC base pairs in the anticodon stem7, 18, 19
. Additionally, we analysed other
members of the translational apparatus which play a role in i-tRNA selection, such as the other initiation
factors (IF1 and IF2), the C-terminal tails of ribosomal proteins uS9 (encoded by rpsI) and uS13 (encoded by
rpsM) which directly interact with the i-tRNA, uS12 which is an interacting partner of IF3, SD-aSD
interactions which affect fidelity of i-tRNA selection and 16S rRNA residues (G1338 and A1339) which
interact directly with the anticodon stem of i-tRNA. Furthermore, we investigated how these mycoplasmal
features may help us understand translation initiation with the unusual AU/GC/GU i-tRNA in E. coli.
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Results
Start codon usage in mycoplasmal species
The mycoplasmal species sustaining on AU/GC/GU i-tRNAs may have a translational apparatus
adapted to suit initiation with the non-canonical i-tRNAs. Such a system might also influence start codon
usage. Therefore, an analysis of the earlier data20
was carried out and it indicates that among the species
having more than 10% non-AUG start codons in their genomes, 75% belong to the AU/GC/GU group. As the
genome sequences of several mycoplasmas are now available, we obtained genome sequences of 12
Mycoplasma species (M. ovis, M. parvum, M. haemominutum, M. pneumoniae, M. genitalium and M.
gallisepticum from the AU/GC/GU group and M. fermentans, M. bovis, M. mobile, M. capricolum, M.
putrefaciens and M. synoviae from the GC/GC/GC group) and used them to demarcate ORFs as described in
Materials and Methods. In agreement with the previous studies, our analyses show that most of the species
from the AU/GC/GU group use a higher percentage of non-AUG start codons (GUG, UUG, CUG, AUA,
AUC, AUU, UUA, AAA, CCU, ACG) than the GC/GC/GC group (Fig. 3). Subsequently, we carried out
computational analyses of the primary sequences of various translational components.
Distinctive features of initiation factors (IF1, IF2 and IF3) in accommodation of i-tRNA with
AU/GC/GU sequence
Sequences for IF1 could not be obtained for many mycoplasmal species rendering their analyses
intractable; and for IF2 sequences, we did not observe any significant trends. In contrast, multiple sequence
alignment of IF3 sequences obtained from NCBI using Clustal Omega revealed many polymorphisms at
important positions. However, the polymorphisms which were consistent for all the AU/GC/GU i-tRNA
containing species were found at the positions R131 (R131P/Y/F) and E134 (E134T/L/M/V/I) (E. coli
numbering) which are otherwise conserved (Table 1, Fig. 4). The R131P mutation in E. coli IF3 (infC135) is
a well-studied allele which was isolated as a suppressor of a start codon mutation of recJ21, 22
, and has been
implicated in the loss of its fidelity. Subsequently, the infC135 was found incapable of discrimination against
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anticodon stem mutants of i-tRNA23
. Therefore, in Mycoplasma species such as M. ovis, M. pneumonia, M.
genitalium etc, the IF3 R131 polymorphisms may exist to allow sustenance of the organism on the non-
canonical AU/GC/GU i-tRNA.
Analysis of mycoplasmal uS9 and uS13
The R131P mutant of IF3 is characterized by an overall loss of fidelity due to deficient discrimination
against P-site binding of tRNA, start codon selection, initiation from leaderless mRNAs and with internal
start codons in the absence of SD-aSD interactions. It is, therefore, possible that the Mycoplasma species with
IF3 R131 polymorphism may harbor other genomic variations to compensate for the compromised activity of
IF3. A well-studied protein involved in i-tRNA discrimination at the P site is the ribosomal protein uS9. In
the crystal structure of T. thermophilus ribosomes, the C-terminal tail of the uS9 protein contacts the i-tRNA
at positions 33 and 346. The C-terminal tail sequence (SKR) of uS9 is also highly conserved amongst bacteria
and its deletion leads to a modest decrease in cellular growth at 37 °C, but significant increase in cold
sensitivity and a decrease in i-tRNA binding to the 30S ribosome12
. Additionally, in vivo studies from our
group have suggested that the uS9 C-terminal SKR sequence decreases P-site binding of anticodon stem
mutants of i-tRNAs11
.
In the multiple sequence alignment of uS9 sequences from numerous Mycoplasma species, we noted
that the species that possessed AU/GC/GU i-tRNAs also harbored an S128T variation in uS9 (Fig. 5),
resulting in the change of conserved SKR tail of uS9 to TKR tail. Further, multiple sequence alignment of
uS13 sequences revealed that the mycoplasmal species sustained on the AU/GC/GU i-tRNA also possessed
longer uS13 tails ending in IESK, IETR or IEGKK sequences (Fig. 6). M. conjunctivae and Aster yellows
witches’ broom phytoplasma with GC/GC/GU containing i-tRNA are exceptions in that they also possess
long uS13 tails. T. thermophilus crystal structures have indicated that the 118th
or final residue of uS13
contacts G29 of i-tRNA which is the first G of the universally conserved 3GC base pairs6. Therefore, the C-
terminal tail of uS13 may have a role in anticodon stem discrimination. Although the uS13 tail tolerates more
variability than the uS9 tail, it generally possesses basic residues which interact with i-tRNA. Deletion of 5
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amino acids of the uS13 tail has no effect on growth of the cell which only slows at the deletion of 36 amino
acids12
. However, the binding affinity of the 30S subunit to all tRNAs is affected in the absence of even 5
amino acids from the C-terminal tail of uS13 (uS13Δ5). This is distinctly different from the phenotype of uS9
protein with a deletion of three amino acids from the C-terminus (uS9Δ3), because the uS9 tail displays
specificity towards certain tRNAs such as the i-tRNA. The uS13Δ5 can rescue the cold sensitivity conferred
by uS9Δ3, indicating the complementary effects of the uS9 and tailed uS13. However, the effects of
lengthening the C-terminal tail of uS13 have not been studied.
Effect of uS9 and IF3 mutations on the growth of E. coli
The computational analysis revealed R131P allele of IF3, known as a relaxed fidelity allele23
, as a
unique feature of mycoplasmal species harboring AU/GC/GU i-tRNAs. It would seem unusual that a relaxed
fidelity allele would be selected without a specific reason. Besides, in the light of our observation of genetic
interaction between the C-terminal tail of uS9 and the 3GC base pairs in the anticodon stem of i-tRNA11
, the
co-occurrence of S128T change in the tail of uS9 in the same group of mycoplamas is also intriguing. Thus,
to investigate the importance of co-occurrence of uS9 and IF3 variations, we generated an uS9 TKR (rpsI
TKR::kanR) mutation in E. coli and combined it with the infC135 (IF3 R131P) mutation
24. We then generated
E. coli strains that lacked chromosomal copies of i-tRNA genes (metZWV and metY) by sustaining them on
plasmid-borne AU/GC/GU mutant i-tRNA (pmetYAU-GU) or wild-type (GC/GC/GC) i-tRNA (pmetY) genes.
The strains also possessed the uS9 TKR and IF3 R131P mutations. In the strain wild type for IF3,
introduction of uS9 TKR afforded enhanced growth (compare curves 1 and 2 in Figs. 7 (i) and 7 (ii)). It was
also observed that for the strains sustained on pmetY (wild type i-tRNA), simultaneous introduction of uS9
TKR/ IF3 R131P mutations resulted in slower growth (Fig. 7 (i), curve 4) than the strain with single mutation
of IF3 R131P (Fig. 7 (i), curve 3). However, when the strains were sustained on the pmetYAU-GU (encoding
AU/GC/GU i-tRNA), the growth difference between the strains with single IF3 R131P (Fig. 7 (ii), curve 3)
and double uS9 TKR/ IF3 R131P (Fig. 7 (ii), curve 4) mutations is diminished. This may suggest that the
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presence of the uS9 TKR mutation is compatible with the IF3 R131P mutation in the presence of the
AU/GC/GU i-tRNA.
Effects of IF3 R131P and S9 S128T mutations on initiation
To investigate the specific effect of the R131P IF3 and S128T uS9 mutations on initiation with the
AU/GC/GU i-tRNA, we made use of our in vivo assay system wherein we use CATam1 reporter having UAG
initiation codon. In this assay, when a plasmid borne copy of the CATam1 reporter (pCATam1) is introduced
into E. coli, it fails to produce chloramphenicol acetyltransferase (CAT). However, when pCATam1 also
harbors metYCUA gene encoding i-tRNA with CUA anticodon (as opposed to CAU) it results in CAT
production providing a measure of the initiation activity of the i-tRNA17, 25
. This reporter system allows
introduction of specific mutations in metYCUA to assess their effects on the initiation activity of the encoded i-
tRNAs. Hence, we mutated the GC/GC/GC sequence of metYCUA to AU/GC/GU and, as a control, to
UA/CG/AU to generate metYCUA/AU-GU and metYCUA/3GC mutant i-tRNA genes, respectively. The
pCATam1metYCUA, or pCATam1metYCUA/AU-GU or pCATam1metYCUA/3GC reporters were introduced into the
parent strain (wild type), or its derivatives harboring IF3 R131P and S9 TKR mutations in singles or together,
to assess the initiation activities of the i-tRNA mutants.
Initiation activities with metYCUA (wild type for GC/GC/GC, and serving as the wild type i-tRNA
control), using the pCATam1 reporter, remained largely unchanged when the uS9TKR or infC135 mutations
were incorporated into the parent strain (Fig. 8A (iii)). However, with uS9 TKR, there was a decrease in
initiation activity (compared to wild type uS9) to about half with the mutant i-tRNAs metYCUA/AU-GU (Fig. 8A
(i), compare bars 1 and 2) and a remarkable decrease in initiation with metYCUA/3GC, a tRNA that lacks all the
three GC pairs in its anticodon stem (Fig. 8A (ii), compare bars 1 and 2). The presence of IF3 R131P
mutation (rpsI SKR infC135) in the parent background (rpsI SKR), caused a remarkable increase in initiation
with metYCUA/AU-GU (Fig. 8A (i), compare bars 1 and 3) and metYCUA/3GC i-tRNA (Fig. 8A (ii), compare bars 1
and 3). Interestingly, the initiation activity of the metYCUA/AU-GU and metYCUA/3GC tRNAs supported by IF3
R131P was significantly decreased by the presence of the uS9 TKR mutation (Fig. 8A (i) and (ii), compare
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bars 3 and 4). However, the levels of initiation with mutant i-tRNAs are still more in the IF3 R131P/ uS9
TKR double mutant than in the strain wild type for IF3 and uS9 (Fig. 8A (i) and (ii), compare bars 1 and 4),
indicating that the uS9 TKR polymorphism in Mycoplasma species only serves to restrict but not eliminate
the increased initiation with AU/GC/GU i-tRNA by the IF3 R131 variant.
We then decided to measure the combined effect of initiation with various start codons in the
background of uS9 and IF3 mutations with pCATAUG and pCATAUA reporter plasmids (i. e. in the presence of
chromosomally encoded i-tRNA genes). Initiation with the AUG start codon between the wild type strain and
its uS9 TKR counterpart (Fig. 8B, compare bars 1 and 3) was not different. However, the infC135 mutation
led to an increase in AUG initiation (Fig. 8B, compare bar 1 with bars 5 and 7). The uS9 TKR mutation has
no discernible effect on initiation with the non-canonical AUA start codon (Fig. 8B, compare bars 2 and 4).
As expected from earlier studies23
, in the presence of the infC135 mutation, AUA initiation increased ~175-
fold (Fig. 8B, compare bars 2 and 6). However, this increase was mitigated (by about half) with the
simultaneous presence of the uS9 TKR mutation (Fig. 8B, compare bars 6 and 8). Once again, we see that the
relaxation (deficiency) of fidelity of initiation triggered by IF3 R131P is partially restricted by uS9 TKR.
Effect of elongated uS13 C-terminal tail on initiation with mutant i-tRNAs
Since we were unable to generate genomic uS13 variants with longer C-terminal tails, we used a uS13
deletion strain KL16ΔrpsM::kan referred to as KL16ΔS13 (a kind gift from Prof. Rachel Green) and
overexpressed either the wild type uS13 or mutant uS13 with an elongated C-terminal tail (uS13 tailed). We
observed that E. coli KL16ΔrpsM::kan grew much poorer than the wild type strain (Fig. 9A, compare curves
1 and 2). Both uS13 and tailed uS13 partially rescue the growth of KL16ΔrpsM (Fig. 9A, compare curves 3
and 4 with 2). Interestingly, towards the stationary phase we see that KL16ΔrpsM grows poorer in the
presence of tailed uS13 than in the presence of uS13 (Fig. 9A, compare curves 3 and 4).
We then investigated the effect of the extended C-terminal tail of uS13 on initiation with the
AU/GC/GU mutant i-tRNA (metYCUA/AU-GU). We see that in log phase, the presence of the longer C-terminal
tail does not affect initiation with the mutant or wild type i-tRNAs (Fig. 9B i, ii, and iii, bars 1 and 2).
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However, in the absence of the uS13 protein, there is a six-fold increase in initiation with the AU-GU mutant
i-tRNA (Fig. 9B (i), compare bars 2 and 3). Interestingly, in stationary phase, the presence of a longer uS13
tail leads to an increase in initiation with the AU-GU mutant i-tRNA as compared to wild type uS13 (Fig. 9B
(iv), compare bars 1 and 2) and an even greater increase in initiation with the 3GC mutant i-tRNA (Fig. 9B
(v), compare bars 1 and 2). However, initiation with metYCUA with a wild type anticodon stem is unaffected
by the longer uS13 tail (Fig. 9B (vi), compare bars 1 and 2), indicating that the observations regarding
AU/GC/GU and the 3GC mutant i-tRNAs are not a consequence of plasmid copy number variation.
Therefore, from our studies it appears that a longer uS13 tail leads to higher levels of initiation with anticodon
stem mutant i-tRNAs only at stationary phase. This may be because of differential incorporation of the uS13
protein with longer tail at stationary phase (as opposed to log phase).
Discussion
Our computational studies have shown that the mycoplasmal species, which possess the AU/GC/GU i-
tRNA variant also have numerous concomitant genetic polymorphisms, some of which influence initiation
with the i-tRNA variants, in E. coli. The IF3 R131P polymorphism as also the presence of an elongated uS13
C-terminal tail (at stationary phase) leads to heightened initiation with the AU-GU i-tRNA, while the
presence of the uS9 TKR mutation curtails initiation with the AU-GU i-tRNA. Therefore, we propose that the
IF3 and uS13 variations in the AU/GC/GU mycoplasma group may have evolved to accommodate initiation
with the unusual AU/GC/GU i-tRNA, while the polymorphism in uS9 may have coevolved to curtail the
deleterious effects of excessive relaxation of translational fidelity. Additionally, our studies in E. coli are the
first to show a functional interaction between the C-terminal tail of uS9 and IF3, whereby a mutation in the C-
terminal tail of uS9 was able to partially rescue the fidelity defects of an IF3 mutant strain.
While we studied the roles of IF3, uS9 and uS13 in mycoplasmal initiation fidelity using our assay
systems, we also considered additional translational features, which may have coevolved to affect
translational initiation with the AU/GC/GU i-tRNA. For instance, the ribosomal protein, uS12 serves to
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modulate translocation of mRNA-tRNA complex through the ribosome26
and it is also one of the interacting
partners of IF3. On aligning mycoplasmal uS12 sequences, we noted that residue 53 (E. coli numbering) is K
(as opposed to R) in species with AU/GC/GU tRNAs (Fig. S1). R53A mutation in uS12 of E. coli leads to
hyper-accurate ribosomes which are resistant to the miscoding effects of paromomycin27
. However,
mollicutes have undergone years of AT-directed evolution, leading to the emergence of genomes with very
low GC content28
. Thus, there is a preponderance of lysine (codons: AAA, AAG) as opposed to arginine
(AGA, AGG, CGN)28
in mycoplasmal genomes. Therefore, it is possible that the AU/GC/GU group is simply
more evolved in the quest for a genome with higher AT content. The 16S rRNA residues G1338 and A1339
form A-minor interactions with base pairs 30--40 and 29--41 in the anticodon stem of P-site bound i-tRNA
and these interactions serve an important function in i-tRNA discrimination in the presence of IF36, 10
. Since
variations of the conserved 3GC base pairs are found in mycoplasma, we wanted to verify that the residues
G1338 and A1339 were conserved in mycoplasmal species as well. From our sequence alignments, it was
evident that G1338 and A1339 remained intact in species from both the AU/GC/GU and the GC/GC/GC
groups (Fig. S2).
It has been shown from our group that the presence of an extended SD-aSD interaction leads to
increased initiation with anticodon stem mutants of i-tRNAs13
. Further, the ribosomal protein S1 which
recognizes the SD sequence of mRNAs (reviewed in 1) and whose absence has been implicated in increased
translation with leaderless mRNAs29
, is missing in most mycoplasmal species30
. The absence of S1 (except in
M. pulmonis31
) is likely to make mycoplasmal species better suited to translation with leaderless mRNAs.
Therefore, we decided to study the characteristics of SD sequences present in our representative Mycoplasma
species. We demarcated ORFs, aSD (Fig. S3) and subsequently SD sequences of 12 representative
Mycoplasma species as described in Materials and Methods. In the AU/GC/GU group, around 34% of the
genes had SD sequences (Fig. S4, grey bars). However, among the mycoplasmas with canonical i-tRNAs
(GC/GC/GC), around 68% of the genes had SD sequences (Fig. S4, green bars). Thus, there was a twofold
difference in the frequency of usage of SD sequences. In the strains with the AU/GC/GU i-tRNA variant,
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12
there is likely to be a great deal of competition with the elongator tRNAs due to the lack of the conserved
GC/GC/GC base pairs (which would ordinarily strengthen selection of the i-tRNA at the P site). It is likely
that more genes do not have SD sequences to allow for greater scrutiny at the P-site and accurate selection of
the AU/GC/GU i-tRNA.
The sequence AU/GC/GU (as opposed to GC/GC/GC) is symptomatic of AT-driven evolution.
However, the other variations in the translation apparatus are not unanimously indicative of AT-driven
change (Table 2). In the case of IF3 R131P/F/Y, which is probably the most influential variation, the changes
to F and Y increase AT-content of the codon, but not the change to P. Similarly, the uS9 S128 residue
changes to T in the AU/GC/GU group is also not AT-driven. We postulate that the initial change of anticodon
stem sequence of i-tRNA (from GC/GC/GC to AU/GC/GU) may have been AT-driven but the subsequent
changes to the regulatory elements of translation were probably adaptive mechanisms to allow initiation with
the AU/GC/GU i-tRNA without a complete loss of overall translational fidelity. It is interesting to note that
the mutations of IF3, uS9, and uS13 affect initiation with the 3GC mutant i-tRNA more significantly than
with the AU-GU mutant i-tRNA. This might suggest that the evolution of the mycoplasmal translational
apparatus which accommodates initiation with the AU/GC/GU variant i-tRNA may also allow initiation with
elongator tRNAs. Initiation with elongator tRNAs alone has been shown to be possible under conditions of
depletion of i-tRNAs and this has been predicted to lead to greater proteome diversity32
. This sort of relaxed
regulation may eventually give rise to an increased proteomic diversity which would be highly conducive to
further evolution.
We recreated some of the mycoplasmal features in E. coli to study initiation with the AU/GC/GU i-
tRNA, and observed that the IF3 R131P mutation allows an increase in initiation with the AU/GC/GU i-
tRNA variant and the non-canonical start codon AUA but the accompanying overall loss of fidelity may be
restricted by the uS9 S128T mutation. However, the combination of uS9 and IF3 mutations still
accommodates initiation with mutant start codons and mutant i-tRNAs more efficiently than a wild type
strain. Also, in stationary phase, the presence of a longer uS13 tail leads to an increase in initiation with the
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13
AU/GC/GU mutant i-tRNA and an even greater increase in initiation with the 3GC mutant i-tRNA.
According to a phylogenetic tree based on whole genome analyses by the Xiao group, M. genitalium, M.
gallisepticum, M. penetrans and M. pneumoniae cluster together in the same clade (clade V) which is the
human-infecting lineage33
. M. gallisepticum is an exception as it infects poultry but it is also under the
strongest selection pressure in the clade indicating evolutionary flexibility and a potential to adapt to new
environments. The Ureaplasma species clustering together in clade I are also the agents of human infection.
The Ureaplasma genus is especially interesting because it accommodates initiation with the AU/GC/GU i-
tRNA with an intact Arg at position 131, indicating the involvement of other genetic variations to
accommodate this unusual i-tRNA. Since all members of clades I and V are also species which are sustained
on AU/GC/GU i-tRNAs, future investigations into the translational machinery of these mycoplasmal species
are imperative.
Material and Methods
Materials
Chemicals, Enzymes and Radioisotopes
Media components were obtained from BD Biosciences (DifcoTM
, USA) or HiMedia (India). The enzymes
used in various nucleic acid restriction and modification procedures were a product of Finnzymes (Finland),
New England Biolabs (USA), Roche (Germany), Promega (USA), GE Healthcare (UK) or Bangalore Genei
(India). Chemicals (molecular biology/ analytical grade) were from Sigma (USA), GE Healthcare or
Qualigens (India). Antibodies were procured from Merck Millipore (Germany). Radioisotopes were obtained
from Board of Radiation and Isotope Technology (BRIT, India) or American Radiolabeled Chemicals Co.
Pvt. Ltd (USA). DNA oligomers were synthesised by Integrated DNA Technologies (USA) or Sigma-Aldrich
(India). DNA sequencing was done at Macrogen (S. Korea).
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14
DNA oligomers, bacterial strains and plasmids
These are listed in Tables 3, 4 and 5 respectively.
MethodsBacterial growth and culturing conditionsE. coli and its derivatives were grown in LB and LB agar
plates (Difco). Media were supplemented with ampicillin (Amp, 100 μg/ml), chloramphenicol (Cm, 30
μg/ml), kanamycin (Kan, 25 μg/ml), or tetracycline (Tet, 7.5 μg/ml) as required.
Growth curve analysis
Growth curve analysis was done by taking four independent colonies of each strain (as specified). They were
grown to saturation in LB with appropriate antibiotics at 37 °C and diluted in LB medium. Aliquots (200 μl)
of the diluted culture were taken in honeycomb plates and shaken in automated Bioscreen C growth readers
(Oy Growth, Helsinki, Finland) maintained at 37 °C temperature. The OD600 was measured at 1 h intervals,
and data were plotted as mean ± standard error of mean.
Genetic manipulations of E. coli
E. coli cells were made transformation competent by the rubidium chloride method and transformation was
carried out by heat shock method34
.
Generation of uS9 mutants
The uS9 TKR mutant strain and a control strain with wild type uS9 linked to the kanR cassette were generated
by the method described in 24
. Briefly, the kanR cassette from pKD4 was amplified with S9 SKR Fp (for
KL16 rpsI SKR::kanR) or S9 TKR Fp (for KL16 rpsI TKR::kan
R) and S9Δ3 Rp. The PCR product was
purified from agarose gel and electroporated into KL16/ pKD46. The strain was validated by PCR with S9 Fp
and S9 Rp. The PCR conditions were, 94 °C for 5 min followed by 30 cycles of 94 °C 1 min, 68 °C 40 s, 72
°C 2 min 40 s followed by a final extension of 72 °C 10 min.
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15
Preparation of cell-free extracts and CAT assays
Cell free extracts were prepared as described 18
and their protein contents were quantified by Bradford’s
assay35
. Chloramphenicol acetyltransferase assays were carried out from four independent colonies11, 14
and
the mean values were plotted, with standard errors.
Bioinformatic analyses
Multiple sequence alignment (MSA) was carried out using Clustal Omega and visualised using Jalview
2.9.0b2. For identification of anti-Shine Dalgarno (aSD) sequences from genomes of Mycoplasma species,
16S rRNA sequences were downloaded from NCBI and BLAST was run against various genomes. Genomic
position of RNA was mapped and aSD sequence core motif (CCUCCU) was found in RNA. Subsequently,
aSD sequence for each organism was marked. For the identification of Shine Dalgarno motifs, ORFs and
whole genome sequences were downloaded from NCBI. Each ORF on the genome was mapped and the
region -7 to -15 nucleotides upstream from the start position (probable SD stretch) was extracted. The
sequence was aligned with aSD sequence of the same organism in all possible frames. Stacking energy36
was
calculated for all consecutive pairs. The lowest energy frame was selected. [12 nucleotide long, energy cutoff
-4.4 kcal/mol37
] The SD position was mapped on the mRNA, to find the distance from the start codon.
Disclosure of potential conflicts of interest:
No potential conflicts of interest were disclosed.
Acknowledgements
We thank our laboratory colleagues for their suggestions on the manuscript.
Funding
Department of Biotechnology (DBT), Ministry of Science and Technology; Department of Science and
Technology (DST), Ministry of Science and Technology; DST J.C. Bose Fellowship (to U.V.); The authors
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16
acknowledge the DBT-IISc partnership programme, University Grants Commission, New Delhi for the
Centre of Advanced Studies, and the DST-FIST level II infrastructure supports to carry out this work.
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References
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25. Mandal N, Mangroo D, Dalluge JJ, McCloskey JA, Rajbhandary UL. Role of the three consecutive G:C base pairs conserved in the anticodon stem of initiator tRNAs in initiation of protein synthesis in Escherichia coli. RNA 1996; 2:473-82. 26. Cukras AR, Southworth DR, Brunelle JL, Culver GM, Green R. Ribosomal proteins S12 and S13 function as control elements for translocation of the mRNA:tRNA complex. Mol Cell 2003; 12:321-8. 27. Panecka J, Mura C, Trylska J. Interplay of the bacterial ribosomal A-site, S12 protein mutations and paromomycin binding: a molecular dynamics study. PloS one 2014; 9:e111811. 28. Muto A, Osawa S. The guanine and cytosine content of genomic DNA and bacterial evolution. Proc Natl Acad Sci U S A 1987; 84:166-9. 29. Kaberdina AC, Szaflarski W, Nierhaus KH, Moll I. An unexpected type of ribosomes induced by kasugamycin: a look into ancestral times of protein synthesis? Mol Cell 2009; 33:227-36. 30. Razin S, Yogev D, Naot Y. Molecular biology and pathogenicity of mycoplasmas. Microbiol Mol Biol Rev 1998; 62:1094-156. 31. Chambaud I, Heilig R, Ferris S, Barbe V, Samson D, Galisson F, et al. The complete genome sequence of the murine respiratory pathogen Mycoplasma pulmonis. Nucleic Acids Res 2001; 29:2145-53. 32. Samhita L, Virumae K, Remme J, Varshney U. Initiation with elongator tRNAs. J Bacteriol 2013; 195:4202-9. 33. Liu W, Fang L, Li M, Li S, Guo S, Luo R, et al. Comparative genomics of Mycoplasma: analysis of conserved essential genes and diversity of the pan-genome. PloS one 2012; 7:e35698. 34. Sambrook. Molecular Cloning: A Laboratory Manual. Cold Spring Harbor, NY, 1989. 35. Bradford MM. A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Analytical biochemistry 1976; 72:248-54. 36. Mathews DH, Disney MD, Childs JL, Schroeder SJ, Zuker M, Turner DH. Incorporating chemical modification constraints into a dynamic programming algorithm for prediction of RNA secondary structure. Proc Natl Acad Sci U S A 2004; 101:7287-92. 37. Freier SM, Kierzek R, Jaeger JA, Sugimoto N, Caruthers MH, Neilson T, et al. Improved free-energy parameters for predictions of RNA duplex stability. Proc Natl Acad Sci U S A 1986; 83:9373-7. 38. Hussain T, Llacer JL, Wimberly BT, Kieft JS, Ramakrishnan V. Large-Scale Movements of IF3 and tRNA during Bacterial Translation Initiation. Cell 2016; 167:133-44 e13. 39. Shetty S. Initiation of protein synthesis: Role of the three consecutive GC base pairs in the anticodon stem of initiator tRNAs. PhD thesis, MCB, IISc, 2015. 40. Low B. Formation of merodiploids in matings with a class of Rec- recipient strains of Escherichia coli K12. Proc Natl Acad Sci U S A 1968; 60:160-7. 41. Mangroo D, RajBhandary UL. Mutants of Escherichia coli initiator tRNA defective in initiation. Effects of overproduction of methionyl-tRNA transformylase and the initiation factors IF2 and IF3. J Biol Chem 1995; 270:12203-9. 42. Varshney U, RajBhandary UL. Initiation of protein synthesis from a termination codon. Proc Natl Acad Sci U S A 1990; 87:1586-90.
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Table 1: List of variations found in IF3 of Mycoplasma species with respect to E. coli IF3. Only functionally
important residues of IF3 have been discussed in the table. Important residues
(E. coli numbering) Variations in different Mycoplasma species (when a residue is conserved partially, exceptions have been listed).
Y75 M. parvum (Q), M. ovis (R), M. hemominutum (R)
T102 Not conserved
P162 Not conserved
E134 M. parvum (T), M. haemominutum (L), M. haemofelis (M), Aster yellows witches’ broom phytoplasma (M), Onion yellows
phytoplasma (M), M. gallisepticum (M), M. genitalium (V, M. pneumoniae (V), M. penetrans (I), M. iowae (I), M. pirum (L)
A42 Mostly conserved
G71 Onion yellows phytoplasma (Q), Aster yellows witches’ broom phytoplasma (Q), M. parvum (Q), M. ovis (E), M. hemominutum (L)
D106 Conserved
L111 Not conserved
P176 M. mobile (Q), M. penetrans (S), M. conjunctivae (R), M. hypopneumoniae (R),
M172 Not conserved
R131 M. gallisepticum (F), M. pneumoniae (F), M. genitalium (F), M. penetrans (Y), M. hemofelis (P), M. parvum (P), M. ovis (P), M.
hemominutum (P), M. pirum (F), M. iowae (Y)
Y107 Not conserved
K110 Quite conserved
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Table 2: Analysis of nucleotide polymorphisms in Mycoplasma species.
Molecule Sequence in GC/GC/GC group Sequence in AU/GC/GU group AT-driven change?
i-tRNA GC/GC/GC AU/GC/GU +
IF3 R131 (AGA codon)
P131 (CCU codon) -
F131 (UUU codon) +
Y131 (UAU codon) +
uS9 S128 (UCA codon) T128 (ACU codon) -
uS12 R53 (CGN/ AGA/ AGG codons) K53 (AAA, AAG codons) +
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Table 3: DNA oligomers used in this study.
Oligomer Name Sequence (5’-3’) Reference/ Source
S9 TKR Fp
GTCGGTCTGCGTAAAGCACGTCGTCGTCCGCA
GTTCACCAAACGTTAAGCTTGTGTAGGCTGGA
GCTGCTTCG
39
S9 SKR Fp GTAAAGCACGTCGTCGTCCGCAGTTCTCCAAA
CGTTAAGCTTGTGTAGGCTGGAGCTGCTTCG This study
S9delRp TTTTCGAAAATTGTTTTCTGCCGGAGCAGAAG
CCAACATATGAATATCCTCCTT 11
S9 int Fp GCTGGCTTCGTTACTCGTGA 11
S9 Rp TCTGTCAGGTGGCAGCAAAA 11
S9 Fp GTAACGAGCACAACCACGCG 11
S13 NcoI Fp ATGCCCATGGCCCGTATAGCAGG This study
S13 HindIII Rp AATAAGCTTATTTCTTGATCGGTTTG This study
S13tail HindIII Rp AATAAGCTTATTTCTTGCCTTCAATCTTTTTTTT
CTTGATCGGTTTGC This study
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Table 4: Bacterial strains used in this study. E. coli strain Genotype Reference/ Source
KL16 E. coli K-12, thi1, relA1, spoT1 40
KL16 rpsI TKR::kanR KL16 derivative where an S128T mutation was generated in uS9. This study
KL16 rpsI SKR::kanR KL16 derivative where kanR is inserted downstream of uS9.
This study
KL16 infC135 rpsI TKR::kanR KL16infC135 derivative where an S128T mutation was generated in
uS9.
This study
KL16 infC135 rpsISKR::kanR KL16infC135 derivative where kanR is inserted downstream of wild
type uS9.
This study
KL16 ΔrpsM::kan KL16 derivative where rpsM is replaced by kanR.
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KL16 infC135rpsI TKR
ΔmetY::catΔmetZWV::kan/ pmetY or
pmetYAU-GU
KL16infC135rpsITKR derivative where kanR has been cured and the
genes encoding i-tRNA have been deleted.
This study
KL16 rpsI TKR ΔmetY::catΔmetZWV::kan/
pmetY or pmetYAU-GU
KL16rpsITKR derivative where kanR has been cured and the genes
encoding i-tRNA have been deleted (supported by pmetY or pmetYAU-GU
i-tRNAs, respectively)
This study
KL16infC135 ΔmetY::catΔmetZWV::kan/
pmetY or pmetYAU-GU KL16infC135 derivative where the genes encoding i-tRNA have been
deleted (supported by pmetY or pmetYAU-GU i-tRNAs, respectively)
This study
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Table 5: Plasmids used in this study. Plasmid Details Reference/ Source
pACDH A low copy no. vector with pACYC ori, compatible with ColE1
origin of replication and harboring tetR
.
41
pKD4 AmpR, KanR, kanR marker is flanked by FRT sequences. 24
pKD46 AmpR
, harbors λ Red recombination genes (γ, β and exo)
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pCATAUG Renamed from pCAT2.5 (harbors AUG initiation codon). 42
pCATGUG Initiation codon of pCATAUG mutated to GUG. 11
pCATUUG Initiation codon of pCATAUG mutated to UUG. 11
pCATAUU Initiation codon of pCATAUG mutated to AUU. 11
pCATAUA Initiation codon of pCATAUG mutated to AUA. 11
pCATam1metYCUA pCATam1 with mutant i-tRNA metY harboring CUA anticodon
(metYCUA) 17
pCATam1metYCUA/3GC pCATam metYCUA with additional mutations of 3GC base pairs,
GC/GC/GC to UA/CG/AU. 25
pCATam1metYCUA/AU-GU pCATam1metYCUA with additional mutations of 3GC base pairs,
GC/GC/GC to AU/GC/GU. 15
pACDHS13 Wild type rpsM cloned into the NcoI and HindIII sites of pACDH This study
pACDHS13 tailed Mutant rpsM with a long C-terminal tail cloned into the NcoI and
HindIII sites of pACDH This study
pmetY Plasmid harboring metY. 15
pmetYAU-GU pmetY derivative harboring mutations in the 3GC base pairs,
GC/GC/GC to AU/GC/GU. 15
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Fig. 1: (A) E. coli initiator tRNA (i-tRNA) and mycoplasmal variations in the anticodon stem. (B) Multiple
sequence alignment of i-tRNA from Mycoplasma species. The box marked with a star denotes bases 29--31
and the box marked with a circle denotes 39--41.
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Fig. 2: 30S-IF3-mRNA-tRNA translation pre-initiation complex (PDB ID: 5LMV)38
. The color code is as
follows: i-tRNA: deep blue; mRNA: black; Part of h42 (of 16S rRNA) labelled G1338 and A1339: red; IF3:
gold; S9: green; S12: sienna; S13: magenta; rest of the 30S components: light blue.
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Fig. 3: Translational start codon usage in genomes of Mollicutes as calculated from whole genome analysis
of 12 Mycoplasma species.
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Fig. 4: Multiple sequence alignment of IF3 sequences from different Mycoplasma species, E. coli and R.
leguminosarum. The black boxes highlight the mycoplasmal species which harbor variations at the 131st
residue (E. coli numbering) as demarcated by the red box.
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Fig. 5: Multiple sequence alignment of uS9 sequences from different Mycoplasma species, E. coli and R.
leguminosarum. The black boxes highlight the mycoplasmal species harboring variations at the 128th
residue
(E. coli numbering). The red box demarcates residue 128.
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Fig. 6: Multiple sequence alignment of uS13 sequences from different Mycoplasma species, E. coli and R.
leguminosarum. The black boxes highlight the mycoplasmal species which harbor longer uS13 C-terminal
tails and are sustained on the AU/GC/GU i-tRNA. The red box demarcates the uS13 tails.
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Fig. 7: Growth analysis. Growth of indicated E. coli strains was studied at 37 °C. Overnight cultures grown in
2xYT ampicillin were diluted 100-fold in ampicillin-containing 2xYT and their growth was monitored using
a Bioscreen C growth reader. Five replicates of all strains were studied. The lines join the mean, and the
vertical bars denote the standard deviation.
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Fig. 8: (A) Initiation with 3GC base pair anticodon stem mutants of metYCUA. (B) Initiation with AUG and
AUA codons.
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Fig. 9: (A) Growth analysis. Growth of indicated E. coli strains was studied at 37 °C with (i) 1 mM IPTG or
(ii) No IPTG. Overnight cultures grown in 2xYT tetracycline were diluted 100-fold in tetracycline-containing
2xYT and their growth was monitored using a Bioscreen C growth reader. Four replicates of all strains were
studied. The lines join the mean, and the vertical bars denote the standard deviation. (B) Initiation with 3GC
base pair anticodon stem mutants of metYCUA. The upper panel includes cell extracts made from log phase
cultures while the lower panel includes cell extracts made from stationary phase cultures. Here, AUGU
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denotes initiation with metYCUA/AU-GU, 3GC denotes initiation with metYCUA/3GC and U35/A36 denotes
initiation with metYCUA with a wild type anticodon stem.
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