Aminoglycoside tolerance in Vibrio cholerae engages translational reprogramming associated to queuosine tRNA modification

Louna Fruchard
Anamaria Babosan
Andre Carvalho
Manon Lang
Blaise Li
Magalie Duchateau
Quentin Giai-Gianetto
Mariette Matondo
Frédéric Bonhomme
Isabelle Hatin
Hugo Arbes
Céline Fabret
Guillaume Sanchez
Virginie Marchand
Yuri Motorin
Olivier Namy
Valérie de Crécy-Lagard
Didier Mazel author has email address
Zeynep Baharoglu author has email address

Institut Pasteur, Université de Paris Cité, Unité Plasticité du Génome Bactérien, UMR3525, CNRS, 75015, Paris, France
Sorbonne Université, Collège Doctoral, F-75005, Paris, France
Institut Pasteur, Université Paris Cité, Bioinformatics and Biostatistics Hub, F-75015 Paris, France
Institut Pasteur, Université de Paris, Proteomics Platform, Mass Spectrometry for Biology Unit, UAR2024, CNRS 2000, Paris, France
Institut Pasteur, Université de Paris, Department of Computation Biology, Bioinformatics and Biostatistics Hub, Paris, France
Institut Pasteur, Université Paris cité, Epigenetic Chemical Biology Unit, UMR 3523, CNRS, 75015, Paris, France
Université Paris-Saclay, CEA, CNRS, Institute for Integrative Biology of the Cell (I2BC), F-91198, Gif-sur-Yvette, France
Université de Lorraine, CNRS, Inserm, UAR2008/US40 IBSLor, Epitranscriptomics and RNA Sequencing Core Facility and UMR7365 IMoPA, F-54000, Nancy, France
Department of Microbiology and Cell Science, University of Florida, Gainesville, Florida 32611, United States
University of Florida Genetics Institute, Florida 32611, United States

https://doi.org/10.7554/eLife.96317.1

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Figures and data

V. cholerae Δtgt shows decreased aminoglycoside tolerance.
A. Competition experiments between WT and Δtgt with the indicated antibiotic or oxidant at sub-MIC concentration. NT: non-treated. TOB: tobramycin 0.6 µg/ml; CIP: ciprofloxacin 0.01 µg/ml; CRB: carbenicillin 2.5 µg/ml; PQ: paraquat 10 µM; H₂O₂: 2mM. B. Competition experiments between WT and Δtgt carrying the indicated plasmids. MH: non-treated. CDEF. Survival of exponential phase cultures after various times of incubation (indicated in minutes on the X-axis) with the indicated antibiotic at lethal concentration: 5MIC: 5 times the MIC; 10MIC: 10 times the MIC. G. PMF measurement of exponential phase cultures using fluorescent Mitotracker dye, measured using flow cytometry. H. Neomycin uptake measurement by flow cytometry using fluorescent Cy5 coupled neomycin. I. Competition experiments between WT and Δtgt carrying either empty plasmid (p0), or a plasmid overexpressing tRNA-Tyr with the native GUA anti-codon, or with the synthetic AUA anticodon. The anticodon sequence is indicated (e.g. tRNATyrAUA decodes the TAT codon). NT: non-treated. TOB: tobramycin 0.6 µg/ml. For multiple comparisons, we used one-way ANOVA. **** means p<0.0001, *** means p<0.001, ** means p<0.01, * means p<0.05. ns: non-significant. Number of replicates for each experiment: 3<n<8.

Codon decoding differences for V. cholerae WT and Δtgt. A. to E. Codon specific translation efficiency in WT and Δtgt using 6xcodon stretches inserted in GFP.
Y axis represents the relative fluorescence of a given GFP in Δtgt over the same construct in WT. NT: non-treated; TOB: tobramycin at 0.4 µg/ml. Each specified codon is repeated 6x within the coding sequence of the GFP (e.g. TACTACTACTACTACTAC). For multiple comparisons, we used one-way ANOVA. **** means p<0.0001, *** means p<0.001, ** means p<0.01, * means p<0.05. ns: non-significant. Number of replicates for each experiment: 3<n, each dot represents one replicate.

Differential translation at tyrosine codons evaluated by growth on carbenicillin of mutated β-lactamase reporters.
The catalytic tyrosine at position 103 was tested in its native sequence (TAC), or with the synonymous TAT mutation. A to D. Growth on microtiter plates. Growth was followed by measuring the OD 620 nm every 15 minutes during 800 minutes. CARB was used at 100 µg/ml. A and C: not TOB. B and D: TOB at 0.2 µg/ml (20% of MIC).

Post-transcriptional regulation in Δtgt and Tyr codon usage bias.
A. and B. Volcano plots showing less and more abundant proteins in proteomics analysis (performed in triplicates) in Δtgt compared to WT during growth without antibiotics (A. where MH is the growth medium), or in sub-MIC TOB at 0.4 µg/ml (B.). C. Codon usage bias calculation example with VC1017 rsxA tyrosine TAC and TAT codons. D. to G. Plots showing codon usage bias for genes lists that are up or down in ribosome profiling analysis (performed in triplicates), for codons decoded by tRNAs with Q modification. Each dot represents one gene of the lists.

Post-transcriptional upregulation of RsxA in Δtgt due to a Tyr codon bias towards TAT and toxicity in sub-MIC TOB.
A. rsxA mRNA levels measured by digital RT-PCR. B. Transcriptional expression levels from the rsxA promoter measured by flow cytometry. C. Translational fusion of rsxA to gfp and gfp alone, with differences in codon usage. *** means p<0.001, ** means p<0.01. ns: non-significant. D. Relative OD 620 nm of WT strain carrying either empty plasmid or plasmid overexpressing RsxA comparing growth in sub-MIC TOB divided by growth in the absence of treatment.

Regulation of tgt expression and tRNA Q levels.
A: tgt transcript levels measured by digital-RT-PCR. Y-axis represents relative abundance compared to the non-treated (NT) condition in WT. For multiple comparisons, we used one-way ANOVA (for A. C. E.). **** means p<0.0001, *** means p<0.001, ** means p<0.01. Only significant differences are shown. B. Stringent response induction measured with P1rrn-gfp reporter shown as fluorescence (Y-axis) as a function of growth (X-axis: OD 600 nm). C. Q levels in tRNA enriched RNA extracts, measured by mass spectrometry. D. Northern blot and quantification of Q levels in tRNA^Tyr. The lower band in the gel corresponds to unmodified tRNA^Tyr. The upper band corresponds to Q-modified tRNA-Tyr. Δtgt is the negative control without modification of tRNA^Tyr. Histograms show the quantification of Q-modified tRNA^Tyr over total tRNA^Tyr, as follows: Q-modified tRNA^Tyr/(Q-modified tRNA^Tyr + tRNA^Tyr without Q)= upper band/(upper band + lower band). 2.5 µg of in tRNA enriched RNA extracts were deposited in lanes WT NT, WT TOB and Δcrp. 0.9 µg was deposited in lanes Δtgt. Number of replicates for each experiment: 3

DNA repair after UV irradiation is more efficient in V. cholerae Δtgt.
A and C. Tyrosine codon usage of DNA repair genes A: in V. cholerae. C: in E. coli. Red indicates positive codon usage bias, i.e. TAT bias. Blue indicates negative codon usage bias for TAT, i.e. TAC bias. B and D. Survival of Δtgt relative to WT after UV irradiation (linear scale) B: in V. cholerae. D: in E. coli. For multiple comparisons, we used one-way ANOVA. **** means p<0.0001, ns: non-significant.

Model.
Upon exposure to sub-MIC aminoglycosides, the expression of tgt is up-regulated in V. cholerae and influences the decoding of tyrosine TAC vs TAT codons. This leads to differential translation from transcripts bearing a codon usage bias for tyrosine codons. The rsxA transcript bears a tyrosine codon bias and its translation can be tuned by tRNA Q modification. RsxA is an anti-SoxR factor. SoxR controls a regulon involved in oxidative stress response. When RsxA levels are high, SoxR is increasingly inactivated and oxidative stress response efficiency decreases. It has been previously shown that sub-MIC aminoglycosides trigger oxidative stress in V. cholerae(78). Increasing RsxA levels thus reduces fitness in TOB by hampering efficient oxidative stress response. As a corollary, decreased RsxA would lead to increased expression of the SoxR regulon, which would allow for more efficient response to oxidative stress, and increased fitness in the presence of sub-MIC TOB. We propose that when Tgt/Q levels in tRNA increase, RsxA synthesis is low and active SoxR levels are high, facilitating the bacterial response to aminoglycoside dependent oxidative stress.

No effect of rluF deletion on fitness in V. cholerae WT and Δtgt strains.
In vitro competition experiments of V. cholerae WT and mutant strains in the absence or presence of sub-MIC aminoglycosides tobramycin TOB and gentamicin (GEN) (50% of the MIC, TOB 0.6 μg/ml, GEN 0.5 µg/ml). MH: no antibiotic treatment. The Y-axis represents log₁₀ of competitive index calculated as described in the methods. A competitive index of 1 indicates equal growth of both strains. The X-axis indicates growth conditions. For multiple comparisons, we used one-way ANOVA on GraphPad Prism. **** means p<0.0001, * means p<0.05. Number of replicates for each experiment: 3<n<10.

Impact of tRNA overexpression on fitness during growth in sub-MIC TOB.
A. Absence of tgt does not visibly affect endogenous tRNA-GUN levels. qRTPCR. A: relative tRNA abundance in Δtgt compared to WT strain in the absence of treatment (NT) and in the presence of sub-MIC tobramycin (TOB). B. In vitro competition experiments between V. cholerae WT and Δtgt strains, carrying a plasmid overexpressing the indicated tRNA; in the absence (NT) or presence of sub-MIC tobramycin (50% of the MIC, TOB 0.6 μg/ml). NT: no antibiotic treatment. The Y-axis represents log₁₀ of competitive index calculated as described in the methods. A competitive index of 1 indicates equal growth of both strains. The X-axis indicates which tRNA is overexpressed, from the high copy pTOPO plasmid. The anticodon sequence is indicated (e.g. tRNA^Tyr_AUA decodes the TAT codon). The following tRNAs-GUN are the canonical tRNAs which are present in the genome, and modified by Tgt: Tyr_GUA, His_GUG, Asn_GUU, Asp_GUC. The following tRNAs-AUN are synthetic tRNAs which are not present in the genome: Tyr_AUA, His_AUG, Asn_AUU, Asp_AUC. tRNA^Phe_GAA is used as non Tgt-modified control. p0 is the empty plasmid. For multiple comparisons, we used one-way ANOVA on GraphPad Prism. **** means p<0.0001, * means p<0.05. Number of replicates for each experiment: 3<n<8. In A, only significant differences are indicated. ns means non-significant.

Post-transcriptional upregulation of RsxA in Δtgt due to a Tyr codon bias towards TAT and toxicity in sub-MIC TOB. ABC.
Translational fusion of TAC and TAT versions of rsxA to gfp (A. 4 hours exponential phase cultures, B. overnight stationary phase cultures). DEF. TAC and TAT versions of gfp alone (C. 4 hours exponential phase cultures without antibiotics, D. in the presence of sub-MIC TOB), measured by flow cytometry. Y-axis represents mean fluorescence. C and F show representative examples of fluorescence observed with indicated reporters.

rsxA levels impact growth in the presence of sub-MIC TOB.
ABCD. Growth curves in microtiter plate reader, in V. cholerae in indicated conditions. P-tgt+: pSEVA expressing tgt. P-rsx+: pSEVA expressing rsxA. P-control: empty pSEVA. E. Growth curves in microtiter plate reader, in E. coli WT and Δtgt in MH or in the presence of tobramycin at the indicated concentrations (in µg/mL). F. Left: Competition experiments in E. coli, with indicated strains. Right: Relative OD 620 nm of indicated strain comparing growth in TOB (0.4 µg/ml) divided by growth in the absence of treatment.

Q detection and quantification by IO4^- oxidation coupled to deep sequencing. The Y-axis represents deletion score, which correlates with the Q34 level in tRNA. Results for tRNAs His, AsnGUU2 and Asp are shown. Analysis was performed for three biological replicates (shown as colored dots) and at least two technical replicates for each strain (only mean of technical replicates is shown). p-values are calculated by two-tailed T-test, error bars correspond to standard error of the mean.

Codon usage.
A and B: Tyrosine codon usage in A: V. cholerae and B: E. coli in the whole genome and selected groups of genes. Red indicates positive codon usage bias, i.e. TAT bias. Blue indicates negative codon usage bias for TAT, i.e. TAC bias. CDE. Gene ontology enrichment analysis in V. cholerae of C: overrepresented gene categories with TAT usage bias. D: underrepresented gene categories with TAT usage bias. E: overrepresented gene categories with TAC usage bias.

Proteomics identify differentially abundant proteins

Proteomics identify differentially abundant proteins

Ribosome profiling.

Ribosome profiling.

RNA-seq V. cholerae WT/Δtgt, in MH and TOB. Only significant differences higher than 2-fold are shown.

RNA-seq V. cholerae WT/Δtgt, in MH and TOB. Only significant differences higher than 2-fold are shown.

Primers, plasmids and strains

Primers, plasmids and strains

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