Abstract
Hydrogen sulfide (H2S) is a ubiquitous gaseous molecule that is endogenously produced in both eukaryotes and prokaryotes. Its role as a pleiotropic signaling molecule has been well characterized in mammals1,2. In contrast, the physiological role of H2S in bacteria only recently became apparent; H2S acts as a cytoprotectant against antibiotics-induced stress and affect the cell’s ability to maintain redox homeostasis 3-5. In E. coli, endogenous H2S production is primarily dependent on 3-mercaptopyruvate sulfurtransferase (3MST), encoded by mstA, previously known as sseA3,4. Here, we show that cells lacking 3MST acquired a unique phenotypic suppressor mutation resulting in compensatory H2S production and tolerance to antibiotics and oxidative stress. Using whole genome sequencing, we mapped a non-synonymous single nucleotide polymorphism (SNP) to uncharacterized Laci-type transcription factor, YcjW. We identified transcriptional regulatory targets of YcjW and discovered a major target, thiosulfate sulfurtransferase PspE, as an alternative mechanism for H2S biosynthesis. Deletion of pspE was sufficient to antagonize phenotypic suppression. Our results reveal a complex interaction between cell metabolism and H2S production and the role, a hithero uncharacterized transcription factor, YcjW, plays in linking the two.
Main
H2S can be generated in numerous pathways-both enzymatically and non-enzymatically and from various substrates beyond cysteine6. The main pathway by which E. coli generate H2S when grown aerobically in nutrient rich LB is via 3MST, encoded by mstA3,4. Phenotypic consequences of decreased H2S production include greater susceptibility to multiple classes of antibiotics and H2O2 3,4,7. However, we discovered that antibiotics-sensitive strain ΔmstA reverted to the resistant phenotype of the isogenic parent when challenged with different antibiotics. The ΔmstA variant, referred to as ΔmstA-sup in this study, was indistinguishable from wild type in time-kill assay analysis and growth curves of cells exposed to gentamicin, nalidixic acid and carbenicillin (Fig. 1a and Supplementary Fig. 1). Furthermore, this strain also had increased tolerance to hydrogen peroxide (H2O2), compared to its still sensitive parent ΔmstA strain (Fig. 1b). Using both the classic lead acetate reactivity test for H2S detection and a fluorescent-based probe, WSP58, we confirmed that this phenotypic reversion was concurrent with increased H2S production, comparable to wild type (Fig. 1c). In contrast, significant levels of H2S remained undetectable in ΔmstA till OD600 1.5.
We utilized whole genome sequencing to identify possible SNPs coding regions that could be responsible for the observed phenotypic suppression. We mapped and validated by PCR a single missense mutation unique to ΔmstA-sup to uncharacterized transcription factor, ycjW. The nucleotide substitution, G to A on the coding strand, results in an amino acid change from serine to asparagine at residue 258 (Fig. 2a).
YcjW is annotated as a putative member of the LacI/GalR family of repressors that are largely responsible for carbohydrate metabolism. Common features of the family include an N-terminal helix-turn-helix DNA-binding domain, a linker domain, and a C-terminal ligand-binding domain 9. To investigate SNP functionality, we constructed two strains, bearing a plasmid expressing either wild type YcjW (pLLY1) or S258N YcjW (pLLSN1), in the background of ΔmstA/ΔycjW. Figure 2b shows that only plasmid-expressed mutated YcjW is able to restore H2S production, quantitated by utilizing the WSP5 probe and qualitatively shown by lead acetate assay. Furthermore, only ΔmstA/ΔycjW;PLL-ycjW (S258N) have an increased survival rate when challenged with gentamicin, H2O2 and nalidixic acid (Fig. 2c and 2d and Supplementary Fig. 2). Thus, we confirm that S258N YcjW in ΔmstA-sup is responsible for the increased hydrogen sulfide production and antibiotics and oxidative stress tolerance relative to ΔmstA.
To identify transcriptional targets of YcjW, we performed ChIP-seq using an antibody against chromosomal 3×FLAG-tagged YcjW from wild type, and ΔmstA cells, and 3xFLAG-tagged YcjW S258N from ΔmstA-sup cells. Figure 3a shows representative peaks identified by MACS210 from aligned sequence reads. The most enriched regions, for all three strains, are at two sites near ycjW; the first site is before the translation start site of ycjM but after a predicted transcription start site and the second lies between ycjT and ycjU. The binding motifs for LacI type family transcription factors are typically palindromes with a conserved central CG pair 11. Recently, Zuo and Stormo experimentally tested the predicted binding motif for YcjW 12. Combined with our analysis of peak summits, we found the same sequence in our data. Using the putative binding sequence, we further restricted peaks to ones containing the conserved 14bp motif, allowing up to three mismatches and with a fold enrichment greater than 5. With those criteria, we identified two additional peaks specifically in ΔmstA, that are not enriched in wild type or ΔmstA-sup. The two sites are near the promoter of narP, encoding a two-component nitrate/nitrite response system and the other is located within the coding sequence of cyaA, encoding ad enylate cyclase (Supplementary Fig. 3).
We then validated transcription factor binding through electrophoretic mobility shift assay (EMSA). We designed 50bp DNA probes containing the predicted binding sequence in the center. The YcjW protein reduced the mobility of the upstream ycjM DNA probe at about a 1:0.5 DNA:protein ratio. Increasing amounts of protein corresponded to an increase in YcjW-DNA complex (Fig. 3b). YcjW (S258N) also reduced DNA probe mobility at the same DNA:protein ratio, using narP probe (Fig. 3c). Titration of the normal protein and S258N YcjW showed that they both bound DNA probe starting at a DNA:protein ratio of 1:0.5. At a ratio of 1:2, no free DNA probe could be detected.
The region downstream of ycjM contains a predicted operon consisting of 10 genes-ycjMNOPQRSTUV and ompG. To test functionality of transcription factor-DNA binding to gene expression, we determined the amount of relative mRNA fold change using qRT-PCR. In ΔycjW, representative genes, ycjM, ycjT, ycjU, and ompG are significantly upregulated, confirming that YcjW is a repressor (Fig. 3d). The absence of YcjW results in constitutive derepression of its regulatory transcriptional targets. The same genes exhibit a similar pattern, increased expression, in ΔycjW;PLL-ycjW S258N relative to wild type MG1655 but not to the extent of its isogenic parent, ΔycjW. Consistent with ΔycjW;PLL-ycjW S258N, those genes are also upregulated in ΔmstA-sup, but not ΔmstA, suggesting that S258N YcjW affects DNA occupancy in vivo but not necessarily in vitro. Mutational analyses of other LacI-TFs have demonstrated that a single amino acid change in the C-terminal can alter effector or co-repressor binding and therefore DNA affinity at target sites 13,14. The SNP is located in the C-terminal effector pocket of the protein, thus raising the possibility that it broadens specificity of inducer recognition, co-repressor binding affinity or oligomerimerization.
qRT-PCR of narP and cyaA showed no significant change in ΔycjW. A small subset of genes regulated by NarP was tested as downstream targets (Supplementary Fig. 4). Two genes, nrfA and ydhU did have a modest increase while two others didn’t. NarP regulation however is complex and involves multiple regulators. Therefore, it is difficult to assess if YcjW-binding upstream of narP and cyaA is functional.
Because many Laci-type repressors act locally in response to some specific effector, we sought to identify the inducer for YcjW by considering its targets. YcjT is homologous to kojibiose phosphorylase from Thermoanerobacter brockii and Pyrococcus sp. Strain ST04 15,16. Kojibiose phosphorylase can reversibly catabolize kojibiose to D-glucose and beta-D-glucose 1 phosphate. The downstream gene, ycjU, has experimentally been shown to encode a beta-phosphoglucomutase 17. Again, utilizing EMSA, we tested to see if kojibiose is the effector molecule for YcjW. The addition of kojibiose at 1mM disrupts the YcjW-DNA complex (Fig. 3e). Other disaccharides tested in excess of up to ten times, trehalose and sucrose, did not affect binding. However, attempts to grow E. coli K-12 MG1655 on minimal media with kojibiose as the sole carbon source were unsuccessful (data not shown and 18). Growth on EZ Rich Defined media supplemented with kojibiose as the carbon source did grow but had a rather pronounced defect. Deletion of ycjW did not improve growth rates either (Supplementary Fig. 5). However, the concentration of kojibiose added to media is limited by its low solubility. It is possible that a higher concentration of kojibiose supplied would support enhanced growth. Taken together, our results indicate that kojibiose might not be the natural inducer of YcjW but perhaps some derivative of kojibiose. Recently, the substrate for YcjM was identified as glucosylglycerate, alongside kojibiose for YcjT 18. Glucosylglycerate is an osmoprotectant in bacteria and archaea and accumulates under salt stress and limited nitrogen availability 19,20. However, most of our experiments were conducted in LB with amino acids constituting the main carbon source. We find it unlikely that synthesis of either the glycoside or disaccharide could occur without the appropriate substrate, and therefore is not likely involved in ΔmstA phenotypic suppression.
While it is not directly evident how a cluster of carbohydrate catabolic genes regulated by YcjW can lead to an alternative pathway for H2S production, pspE encoding a thiosulfate sulfurtransferase, lies immediately upstream of ycjM. PspE has mercaptopyruvate sulfurtransferase activity, albeit low compared to thiosulfate 21. It is part of a cluster of genes known as the phage shock operon, consisting of pspABCDE. Although it can be co-regulated with the other psp genes, it can also be transcribed independently from its own promoter22. PspF is the transcriptional activator and phage shock protein A, encoded by pspA, negatively regulates PspF23.
pspE mRNA expression is significantly increased in ΔmstA-sup and ΔycjW relative to wild type cells. In contrast, there are no significant differences in relative expression of the other two thiosulfurtransferase genes (Fig. 4a). Furthermore H2S production is undetectable during early exponential and mid-log phase in ΔmstA-sup/ΔpspE (Fig. 4b). However, at late logarithmic phase, H2S levels are now detectable to the same degree as MG1655 and ΔmstA-sup. In addition, overnight incubation with lead acetate strips shows no discernable difference in H2S extracellular production between the three strains (Supplementary Fig. 6). We conclude from the significant delay of H2S generation in ΔmstA-sup / ΔpspE that PspE is capable of generating H2S in early growth phases as observed in ΔmstA-sup. However, at later growth stages, another pathway for H2S production is activated and/or PspE is no longer sufficient. Moreover, ΔmstA-sup/ΔpspE also has increased sensitivity to gentamicin treatment compared to ΔmstA-sup and E. coli MG1655 but not quite as sensitive as ΔmstA. Overexpression of PspE in ΔmstA increases survival rate but only to the extent of ΔmstA-sup/ΔpspE, not ΔmstA-sup or wild type (Fig. 4c). Altogether, we conclude that the SNP in ycjW resulted in increased expression of pspE in ΔmstA-sup. This is sufficient but not wholly responsible for increased H2S biosynthesis and in turn, the phenotypic suppression observed in ΔmstA-sup. We propse a model wherein, E.coli cells lacking MstA acquires a SNP in transcription factor YcjW. The SNP imparts moderate constitutive expression of YcjW targets, one of which is pspE. Thiosulfate sulfurtransferase PspE is then able to increase H2S production in ΔmstA, and subsequently protect the cells from antibiotics and H2O2 induced stress (Fig. 4d).
The region upstream of pspE does not contain a strong binding motif for YcjW, nor do the regions flanking regulators PspA and PspF. This is not entirely unexpected since none of the other genes tested in the psp operon were upregulated in ΔmstA-sup or ΔycjW (Supplementary Fig. 6). Additionally, the moderate but significant increase of pspE mRNA in ΔycjW, in comparison to ycjMNOPQRSTUV-ompG, suggests a more complicated interaction than direct DNA-binding. It may be indicative of “leaky” expression driven by the proximity of the 3’end of pspE to predicted transcription start sites for ycjM and the binding site of YcjW. Perhaps, YcjW acts via a co-repressor. Another possibility is that the metabolic state of ΔmstA-sup with mutated ycjW induces pspE as a consequence. And finally, the enzyme(s) that is induced in ΔmstA-sup; ΔpspE, after exponential growth, has not been identified and remains a target for future studies.
Altogether, our results reveal an alternative H2S generator (PspE) that is mobilized as a result of rapid evolutional adaptation to antibacterial stress. The SNP in YcjW, regulating metabolism to at least two rare sugars, presents an interesting link between sulfur metabolism and carbon availability. Moreover, a SNP in YcjW reflects the striking genetic plasticity employed by bacteria to promptly adapt to environmental changes and stimuli and highlights the survival advantage imparted by endogenous H2S.
Methods
General growth conditions
For the general cultivation of E.coli, strains were grown in LB broth supplemented with kanamycin (50ug ml−1), or chloramphenicol (30ug ml−1) as appropriate. Growth on solid medium contained 1.5% agar added to LB. Where noted, MOPS EZ Rich Defined Medium Kit (Teknova) was used in place of LB24. Cysteine solutions were prepared immediately before use, as needed.
Construction of strains and plasmids
For a list of all strains used throughout this work, refer to Table 1.1. BW25112 and its derivatives are from the E. coli Keio Knockout Collection25 (Thermo Scientific). Introduction of new mutations into E.coli MG1655 were achieved through P1 transduction as previously described26. Temperature-sensitive FLP recombinase plasmid pCP20 was used for the excision of selective markers as needed27. All constructs were verified with PCR and sequencing. Primers used throughout this study are listed in Table 1.2.
To generate pLLY1, ycjW was PCR amplified from E.coli MG1655 using primers LL10 and LL11 and cloned into pACYC184 plasmid (NEB) using the Gibson Assembly Mastermix, according to the manufacturer’s protocol (NEB). Plasmid pLLSN3 was generated as above except ycjW was PCR amplified from mstA-sup. The Q5 Site-Directed Mutagenesis Kit (NEB) was used to generate pLLSN1 from pLLY1, according to manufacturer’s protocol.
Transformations were performed using the CaCl2 competent cell protocol28. All plasmids were sequenced for verification.
Addition of 3xFLAG tag to ycjW at its chromosomal locus was achieved as previously described, with slight modifications29. Briefly, primers pLL14 and pLL15 were used to PCR amplify CmR cassette from pKD4. PCR product was transformed into appropriate electrocompetent strains.
H2S detection
End-point detection of H2S production by lead acetate strips were performed as previously described3. Test strips were purchased from Sigma-Aldrich. Monitoring H2S generation with the WSP5 fluorescent probe followed a modified protocol from Peng et al.8 Briefly, cells were grown in LB at 37°C to desired OD600 and aliquots of approximately 4×108 cells were taken. The extinction coefficient used for calculations is OD600 of 1.0 is equal to 8×108 cells. A working solution of WSP5 was made immediately before use and added to cells for a final concentration of 10uM. Samples were incubated at 37°C for 30 minutes and then washed in PBS buffer, pH 7.4, to remove excess probe. Cells were resuspended in PBS buffer and incubated at room temperature for 30 minutes. Cytation3 (Biotek) was used to take fluorescent readings, at excitation 500 nm and emission 533 nm. All experiments were repeated for a total of three times. Background values were subtracted during analysis.
Time-kill assay and growth curves
Overnight cultures of E. coli were diluted 1:300 into fresh media and grown to an OD600 of ~0.2. A 1ml aliquot was serially diluted and plated onto LB agar plates to determine initial colony forming units per ml (cfu ml−1) after overnight incubation at 37°C. Antibiotics were added to the cultures at indicated concentrations. Aliquots of 1ml were collected at specified time intervals, serially diluted and plated. Results from three independent experiments were plotted in GraphPad version 5.0.
Growth curves were generated from Bioscreen C automated growth analysis system as previously described3. Antibiotics were purchased from Sigma-Aldrich or Gold Biotechnology.
Whole genome sequencing
Overnight cultures of E. coli cells were used for genomic DNA isolation. The MasterPure Complete DNA Purification Kit (Epicentre) was used to purify DNA according to the manufacturer’s protocol. DNA samples were quantified using the Quant-IT PicoGreen dsDNA assay kit (Thermo Fisher) according to manufacturer’s protocol. DNA was sheared to appropriate size with Covaris, followed by adaptor ligation. Sequencing was performed at New York University School of Medicine’s Genome Technology Center.
Quantitative RT-PCR
Cells were grown until appropriate OD600 and aliquots were collected and treated with RNAprotect Bacteria Reagent (Qiagen). After 5 minutes, cells were harvested and resuspended in lysis buffer (RNase-free TE buffer, 10 mg ml−1 lysozyme, 100 ug ml−1). Trizol LS (Thermo Scientific) was used according to manufacturer’s protocol to extract total RNA. Samples were treated with DNase (Invitrogen) and purified using spin columns (Zymo Research). Superscript III reverse transcriptase (Invitrogen) was used to synthesize cDNA. qPCR reactions were amplified using Power SYBr Green PCR Master Mix (Applied Biosystems) with appropriate primer sets and cDNA template.
ChIP-seq
ChIP was carried out as previously described with the following modifications30. Briefly, cells were grown at 37°C to OD600 ~0.4 and a final concentration of 1% formaldehyde was added for in vivo cross-linking of nucleoprotein. A final concentration of 0.5M glycine was added to the culture to quench the reaction after a 20 minute incubation. Cells were collected by centrifugation and washing twice with 1X cold Tris-buffered saline then frozen in liquid nitrogen and stored at −80. Cells were resuspended in lysis buffer (50mM Tris [pH 7.5], 100mM NaCl, 1mM EDTA, protease inhibitor [Roche], 10 mg ml−1 lysozyme). After incubation at 37°C, IP buffer (50mM HEPES-KOH, 150mM NaCl, 1mM EDTA, 1% Triton X100, 0.1% sodium deoxycholate, 0.1% SDS, protease inhibitor [Roche]) was added at a 1:3 ratio. DNA was sheared using ultrasonicator Covaris M220 on a 10 seconds on and 10 seconds off cycle for a total of 50 cycles.
The supernatant was incubated with 3xFLAG antibody (Biolegend) and Dynabeads Protein G (Thermo Scientific) overnight at 4°C. Samples were then washed twice with IP buffer, once with IP buffer+500mM NaCl, once with wash buffer (10mM Tris, 250mM LiCl, 1mM EDTA, 0.5% NP-40, 0.5% sodium deoxycholate), and a final wash with TE. Immunoprecipitated complexes were eluted in elution buffer (50mM Tris, 10mM EDTA, 1% SDS) at 65°C for 20 minutes. Samples were treated with RNAse A (Qiagen), at 42°C and then uncross-linked with elution buffer+pronase for 2 hours at 42°C, followed by 6 hours at 65°C. DNA was purified using ChIP Clean and Concentrate (Zymo Research). Prior to sequencing, DNA was checked on TapeStation 2200 for appropriate size (Agilent). ChIP experiments were repeated for a total of three replicates.
For sequencing, sample libraries were prepared by using the NEBNext ChIP-seq Library (Illumina), according to manufacturer’s protocol. Samples were sequenced on NextSeq 500 (Illumina). Bowtie and MACS2 were used for aligning and peak-calling, respectively10.
Electrophoretic mobility shift assay
Protein purification
YcjW and S258N YcjW were cloned into plasmid pet28-SUMO using the Gibson Assembly Mastermix kit, according to the manufacturer’s protocol (NEB). Auto-induction media was used for protein production (152). Cells were harvested and resuspended in lysis buffer (1M NaCl, 5mM Imidaziole, 5% Glycerol, protease inhibitor cocktail [Roche]) and sonicated. AKTA Start system was used for chromatography with HisTrapHP columns (GE Healthcare Life Sciences). Columns were washed in wash buffer (50 mM Tris-Cl [pH 8.0], 10 mM Imidazole, 5% Glycerol, 500 mM NaCl), followed by gradient elution with elution buffer (50 mM Tris-Cl [pH 8.0], 250 mM Imidazole, 5% Glycerol, 250 mM NaCl). The SUMO tag was cleaved with SUMO protease in dialysis buffer (200 mM NaCl, 50 mM Tris-Cl [pH 8.0], 5% Glycerol, 1mM DTT). Samples were applied to a HiTrap HeparinHP column (GE). Columns were washed with buffer (20mM Tris [pH 8.0]. 50mM NaCl, 5% glycerol), and eluted in elution buffer (20 mM Tris [pH 8.0], 1.5 M NaCl, 5% glycerol). The sample was concentrated to 5 mL and injected onto a Superdex 200 column with GF buffer (20 mM Tris-Cl [pH 8.0], 50 mM NaCl, 1 mM DTT).
EMSA
dsDNA probes containing the binding sequence were radiolabeled with gamma 32P rATP using T4 polynucleotide kinase (NEB). Labeled probes were purified by passage through size exclusion columns (Bio-Rad). Binding reactions were done as previously described12. The gel was then exposed to a phosphor screen and visualized on Storm 820 Phosphorimager (GE Healthcare). Experiments with various disaccharides were done in a similar fashion, except purified protein was incubated with appropriate sugar for 20 minutes at room temperature before addition of radiolabeled probe.
Acknowledgments
This work was supported by the NIH grant R01 GM126891, Blavatnik Family Foundation, and the Howard Hughes Medical Institute.