Abstract
Small regulatory RNAs (sRNAs) play a role in the control of bacterial virulence gene expression. In this study, we investigated an sRNA that was identified in Streptococcus pyogenes (group A Streptococcus, GAS) but is conserved throughout various streptococci. In a deletion strain, expression of mga, the gene encoding the multiple virulence gene regulator, was reduced. Accordingly, transcript and proteome analyses revealed decreased expression of several Mga-activated genes. Therefore, and because the sRNA was shown to interact with the 5′ UTR of the mga transcript in a gel-shift assay, we designated it MarS for m ga-activating regulatory sRNA. Down-regulation of important virulence factors, including the antiphagocytic M-protein, led to increased susceptibility of the deletion strain to phagocytosis and reduced adherence to human keratinocytes. In a mouse infection model, the marS deletion mutant showed reduced dissemination to the liver, kidney, and spleen. Additionally, deletion of marS led to increased tolerance towards oxidative stress. Our in vitro and in vivo results indicate a modulating effect of MarS on virulence gene expression and on the pathogenic potential of GAS.
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Introduction
Streptococcus pyogenes (group A Streptococcus, GAS) is a strictly human pathogen that is responsible for a variety of infections of distinct severity1. While superficial infections of the upper respiratory tract and the skin can be treated effectively with antibiotics, invasive streptococcal diseases remain life-threatening. The development of invasive infections and immune sequelae involves at least one or more of the following parameters: insufficient treatment of a primary infection, persistence of streptococci in the host tissue, and the expression of specific virulence factor genes by the bacteria2. Control of virulence gene expression by stand-alone transcription factors and two-component systems are known to play a role in virulence determination in GAS3. An additional level of bacterial gene expression control is provided by small regulatory RNAs (sRNAs)4. Bacterial sRNAs can serve as negative regulators by inhibiting translation or by decreasing mRNA stability and can also function as positive regulators by stabilizing mRNA transcripts or initiating the translation of mRNAs5,6. Although several global sRNA screens have recently been performed in streptococci, the RNA-dependent regulatory network in GAS is not yet well understood7.
Several trans-acting sRNAs, targeting mRNA sequences by direct base pairing, have been discovered in GAS. The pleiotropic effect locus (Pel) was described to have an effect on virulence and to influence the production of several virulence factors, including the M-protein, the cysteine protease SpeB, fibronectin-binding protein, and streptokinase8. The untranslated mRNA of pel, which also contains the gene for the streptolysin S peptide (sagA), was shown to be an effector of virulence factor expression in GAS9. However, in the GAS M1T1 lineage, no regulatory function of PEL could be observed10,11.
The sRNA gene rivX is located downstream of the transcriptional regulator gene rivR. While RivR was shown to affect transcriptional activation by Mga, possibly by interacting with Mga protein, RivX was hypothesized to act through a separate but as yet unknown pathway to increase the expression of multiple genes that are regulated directly or indirectly by Mga12. In a conflicting report, RivR was shown to be a negative regulator of capsule production in GAS while no regulatory function could be assigned to RivX. No influence of the rivR/X locus on the expression of mga or mga-associated genes was detected in this study13.
Until now, the only extensively characterized and functionally validated sRNA in GAS was FasX. FasX acts as positive regulator of the fasBCA operon, coding for the fibronectin/fibrinogen binding/haemolytic activity/streptokinase regulator14. FasX was shown to positively affect streptokinase production by stabilizing ska mRNA15. FasX also acts as a negative regulator of pilus expression by destabilizing the pilus operon mRNA and inhibiting the translation of the cpa transcript, which encodes a minor pilus protein16. By binding to and inhibiting the translation of different mRNAs of the fibronectin, collagen, T-antigen (FCT) region, control over the pilus gene region by FasX varies in a serotype-specific fashion17. In a subsequent report, FasX was shown to negatively control the production of two fibronectin-binding proteins, PrtF1 and PrtF2, encoded by the FCT region18.
In this study, we phenotypically characterize the GAS wild-type strain 591 (referred to as GAS M49 591 throughout the text) lacking the m ga-activating regulatory sRNA (MarS). Employing transcript analyses, proteomics, and a mouse infection model, we show that MarS modulates Mga-dependent virulence factor gene expression, affects capsule production, and influences the fate of GAS in the host. We also show a direct interaction of MarS with the 5′ UTR of the mga transcript using an electrophoretic mobility shift assay (EMSA).
Results
Deletion of marS in GAS 591
Genome-wide screening of the GAS wild-type strain 591 (referred to as GAS M49 591 throughout the text) resulted in an extensive list of candidate sRNA genes19. To identify sRNAs that were potentially involved in pathogenicity of GAS, we focused on sRNA genes that were differentially expressed in different media or throughout growth. Among those, marS (formerly designated sRNASpy490957c) is conserved throughout lactic acid bacteria, and a cis-regulatory function was predicted by a comparative genomics-based study using CMfinder20. However, the sRNA is transcribed independently from adjacent genes in several GAS serotypes10,19,21. Furthermore, in Streptococcus mutans and S. pyogenes, the presence of a terminator sequence and a strong promoter downstream of marS indicates that transcription is terminated prior to the downstream gene, Spy49_0957c, which is transcribed from an independent promoter19,22. A schematic representation of the genomic locus is presented in Fig. 1A. The sRNA gene does not encode a peptide. However, on the antisense sequence of the marS gene, a 108-bp ORF is located, which could lead to the expression of a 35 AA peptide for which no homologues were found by BLAST23 analysis. The stability of the marS transcript, MarS, was determined following rifampicin treatment by RT-qPCR. Transcript stability was high in GAS M49 591 (Fig. 1B), consistent with prior findings obtained in the GAS M1T1 strain MGAS222110. To study the role of MarS, an isogenic deletion strain was constructed and designated ΔmarS. Complementation of the gene deletion was achieved by ectopic expression of the sRNA gene from a shuttle vector under the control of its own promoter (ΔmarS::marS). This strategy helps exclude an influence of spurious mutations introduced during mutagenesis and was recently suggested by Cho24. Furthermore, whole genome sequencing was performed to rule out the occurrence of spontaneous mutations in the recombinant strains. Expression of marS in the respective strains was determined by Northern blot analyses of total RNA isolated from bacteria grown to the exponential phase (Fig. 1C). There was no detectable expression of marS in the deletion strain. By contrast, ΔmarS::marS showed increased expression in comparison to the parental strain, likely due to a higher copy number of the expression vector. These results were verified by RT-qPCR. No PCR product was detected in the RNA sample from ΔmarS, whereas the transcript level in ΔmarS::marS was increased 2-fold in comparison to WT. GAS M49 591 and the recombinant derivatives had similar growth characteristics in THY medium (WT: µ = 1.11 ± 0.09; ΔmarS: µ = 1.09 ± 0.09; ΔmarS::marS: µ = 0.89 ± 0.12). The differences between the strains were not significant (t-test). These data were generated from three independent experiments.
Lack of MarS results in decreased survival of GAS M49 591 in human blood
To investigate the role of MarS in a more pathogenically relevant environment, we assessed the ability of GAS M49 591 WT, the marS deletion mutant, and the marS complementation strain to grow ex-vivo in human blood. ∆marS showed decreased growth in human blood in comparison to WT (Fig. 2A, Fig. S1). In the complementation strain, growth was restored to the WT level. To distinguish whether cellular or non-cellular components of human blood were responsible for the reduced growth of ∆marS, growth in human plasma was assessed. As shown in Fig. 2B and Fig. S2A, growth of ∆marS was not inhibited in human plasma. Consistently, the deletion of marS resulted in a higher susceptibility towards phagocytosis by human neutrophils (Fig. 2C, Fig. S2B). The number of extracellular bacteria was slightly reduced in the marS deletion strain relative to WT (Fig. 2D). Statistical analyses of non-normalized data showed that the decrease of associated bacteria was not significant (Fig. S2C).
MarS positively influences capsule production
The hyaluronic acid capsule of GAS supports evasion of the host immune system through molecular mimicry and confers resistance to phagocytosis25,26,27. Since ∆marS showed decreased growth in human blood and a higher susceptibility towards human neutrophils, we tested whether capsule production is impaired in this strain. No significant difference in hyaluronic acid abundance was detected between ∆marS and the parental strain (Fig. 3A). Interestingly, the complementation strain showed increased hyaluronic acid content in comparison to WT. This observation is in accordance with the higher marS transcript abundance in ΔmarS::marS (Fig. 1C) and suggests a positive effect of MarS on capsule production. To analyse a potential influence of MarS on hasABC mRNA abundance, we measured hasABC transcript abundance by RT-qPCR (Fig. 3B). The gene products of the hasABC operon are responsible for hyaluronic acid synthesis in GAS28,29. ∆marS showed no significant differences in hasABC transcript level in comparison to the parental strain, whereas the complementation strain showed a significantly increased abundance of the hasABC transcripts in comparison to both WT and ∆marS. GAS M49 591 is characterized by a low endogenous level of capsule production28. Thus, the effect of MarS on hyaluronic acid synthesis was investigated in MGAS8232 (serotype M18) (referred to as GAS M18 MGAS8232 throughout the text). The hyaluronic acid production of GAS M18 MGAS8232 was considerably higher than that of M49 (Fig. 3C). The GAS M18 MGAS8232 marS deletion strain showed a reduced capsule production in comparison to both the GAS M18 MGAS8232 WT and the complementation strain GAS M18 MGAS8232 ΔmarS::marS (Fig. 3C). This result indicates a positive regulatory effect of MarS on capsule production in GAS.
MarS influences adherence to human keratinocytes
To test whether MarS influences adherence and invasion, bacteria were incubated with a human keratinocyte cell line (HaCaT). Deletion of marS led to a reduced ability to adhere to HaCaT cells, which was restored in the complementation strain (Fig. 4).
Putative target mRNAs of MarS include mga and hasB
One of the major mechanisms of sRNA-mediated regulation in bacteria is direct binding of the sRNA via base pairing to a target mRNA. Complex formation depends on complementary regions within the RNA sequences and on the respective secondary structures. The IntaRNA30,31 algorithm was employed to predict MarS-mRNA interactions in GAS M49 591. The sequence of S. pyogenes NZ131 (NC_011375.1) served as a reference genome. Among the 28 predicted targets, mga, the gene encoding the multiple virulence gene regulator, was identified with a high probability (Table 1). The putative binding site lies within the 5´untranslated region (5´UTR) of mga (Fig. 5A) and is conserved in serotypes M2, M4, M18, M28, M44, M49, M53, M59, M66, M71, M82, M83, M 87, M89, and M101 as determined by BLAST23 analysis. In silico prediction also identified hasB, encoding the UDP-glucose 6-dehydrogenase, which is part of the capsule synthesis operon in GAS (Table 1). The predicted binding site is located on the hasABC polycistronic transcript at the 3′ end of the hasA coding region (Fig. 5B). For both targets, a common binding site is situated in MarS. The secondary structure of MarS was predicted by RNAfold (The ViennaRNA Web Services, http://rna.tbi.univie.ac.at/) and illustrated using VARNA GUI32 (Fig. 5C).
MarS binds to the 5′ untranslated region of mga
To determine whether MarS binds directly to the 5′ untranslated region of the mga mRNA, we performed RNA-RNA electrophoretic mobility shift assays (EMSAs). A biotin-labeled RNA corresponding to the 5′ end of the mga RNA was incubated with increasing amounts of MarS, which resulted in a shift of the probe to a higher molecular weight complex (Fig. 6, lanes 2-4). To verify the role of the predicted mRNA binding site in MarS (Fig. 5C), we used a mutated form of MarS (mmMarS), in which two residues of the putative binding site were replaced (88-CC-89/88-GG-89). In reactions containing mmMarS, the mga RNA probe was not shifted (Fig. 6, lane 5). The specificity of the binding was confirmed by incubation with increasing concentrations of unlabeled mga RNA, which reduced the shifting (Fig. 6, lanes 6-8).
Deletion of marS results in lower mga and mga-controlled transcript levels
The influence of MarS on the transcript abundance of the putative target mga and virulence factor genes directly regulated by Mga33 was investigated. Total RNA from GAS M49 591 and the recombinant derivatives either grown in THY (Fig. 7A) or following exposure to human blood (Fig. 7B) was analysed by RT-qPCR with primers specific for mga, emm, sclA (streptococcal collagen-like protein), and sof (serum opacity factor). In all cases tested, the abundance of the transcripts was significantly decreased in the deletion mutant compared to that in WT (Fig. 7A/B). In ΔmarS::marS, the phenotype could be restored. Together, these results indicate a positive regulatory influence of MarS on mga and thereby on the expression of genes regulated by Mga. To examine the impact of mga mRNA stability on this effect, the transcript abundance was determined following rifampicin treatment (Fig. 7C). The lack of MarS did not influence mga transcript stability within the first three min. In ΔmarS::marS, mga mRNA stability was slightly improved compared with that in WT and the deletion mutant. The half-life of the mga transcript as calculated by linear regression analyses was 0.57 min in WT, 1.15 min in ΔmarS, and 4.58 min in ΔmarS::marS. Thus, the effects on the Mga regulon in ΔmarS were not caused by reduced mga mRNA stability in the marS deletion strain.
Down-regulation of MarS target gene transcription affects the proteome of GAS M49 591
Given the differential expression of several Mga-controlled genes encoding surface proteins in ΔmarS, we set out to investigate the proteome of the sRNA deletion strain compared with WT and the complementation strain. Cytoplasm-depleted fractions were analysed by nano LC-mass spectrometry. The total number of proteins quantified by at least three and two peptides amounted to 885 and 1001, respectively, representing a high coverage of the proteome (Supplementary Data S1). Seventeen proteins were differentially regulated (a fold change above two) between the investigated strains (Table 2). For the majority of those, differential synthesis could be detected in the exponential (exp), transitional (tra), and stationary (stat) growth phases. Antiphagocytic M protein, fibronectin-binding protein, Fc-gamma receptor, and serum opacity factor, encoded by emm49, sfbX49, Spy49_1672c, and sof, respectively, were reduced in ΔmarS samples compared with those in WT, whereas protein abundance was restored in the complementation strain (Table 2). Mga protein abundance was also reduced in the deletion strain in comparison to WT, but quantification was not meaningful in the cytosol-depleted samples that were used for the analyses. Mga contamination most likely resulted from an interaction with chromosomal DNA hampering complete removal from those samples. Thiol-activated cytolysin (slo) was reduced in ΔmarS during exp and stat. In the complementation strain, the protein level was slightly increased in comparison to WT during tra and stat. Thus, down-regulation of the Mga-controlled gene transcription observed in ΔmarS (Fig. 7A) resulted in a decreased synthesis of the corresponding gene products in the deletion mutant. Furthermore, the collagen-like surface proteins A and B and C5a peptidase were reduced in ΔmarS samples in comparison to WT. The hyaluronic acid synthesis proteins HasA and HasB were increased in ΔmarS::marS, which is in accordance with the increased capsule production by this strain (Fig. 3A). Abundance of the cysteine proteinase SpeB was significantly reduced in both ΔmarS and in ΔmarS::marS in comparison to WT, indicating that these changes were not MarS-dependent. Taken together, of 13 proteins that were down-regulated in ΔmarS compared with those in WT, 10 were known surface-associated or secreted molecules, and two were proteins of unknown function. Although the extracellular ratios of the secreted proteins may differ from the values measured in the cytoplasm-depleted fraction of the cell extracts, their general regulation should be reflected by the data. The protein abundance of the capsule synthesis proteins HasA and HasB was significantly increased in ΔmarS::marS compared with those in WT.
Lack of MarS leads to a greater bacterial dissemination in vivo
To assess the influence of MarS on the virulence of GAS M49 591 in vivo, a mouse infection model was employed. Mice were infected i.p. with 8 × 107 colony forming units (CFUs) GAS M49 591 WT, ΔmarS, and ΔmarS::marS. All animals showed signs of severe bacterial infection and were sacrificed after 24 h. Bacteria were sampled from mouse liver, lung, kidney, and spleen for CFU determination. From the kidneys of infected mice, a significantly greater number of living ΔmarS bacteria could be isolated compared with that in WT and the complementation strain (Fig. 8A). In the liver, significantly more ΔmarS cells were detected than WT cells; in the spleen, the number of ΔmarS::marS bacteria was significantly reduced in comparison to the parental and deletion strains (Fig. 8A). A slightly larger number of ΔmarS was detected in the lungs of the infected mice compared with that of the other two strains, but the differences between the samples were not significant. Thus, in all organs tested, there was a greater number of viable bacteria in the deletion strain than in WT and the complementation strain.
Increased survival of ΔmarS in the host kidney correlates to increased oxidative stress resistance
Reactive oxygen species (ROS)-related DNA damage was measured using a qPCR-based method34. Therefore, total DNA from the kidney and spleen of infected mice, containing host DNA and bacterial DNA, and of PBS-treated controls, containing only host DNA, was isolated. DNA lesions were detected in the mitochondrial DNA (mtDNA) of the host and in the genomic DNA of bacteria using primers specific for the mitochondrial D-loop sequence and the bacterial gyrA, respectively. Infection with any of the three strains resulted in a high level of mtDNA damage in the kidney (≥30 lesions per 10 kb) (Fig. 8B). The differences between the mtDNA damage of the samples collected following infection with the different strains were not significant. In the spleen, which showed a higher bacterial load in this experiment (Fig. 8A), mtDNA damage was less severe than in the kidney (Fig. 8B). Again, no strain-specific differences in mtDNA damage could be detected. Corresponding to the mtDNA data, bacterial DNA isolated from the kidney showed a high level of damage. Bacterial DNA damage was significantly reduced in ΔmarS in comparison to the parental and the complementation strains (Fig. 8C). In contrast, the overall bacterial DNA damage in samples isolated from the spleen was low. DNA from WT cells showed approximately 5 lesions/10 kb, but the difference in comparison to untreated bacteria was not significant (Fig. 8C). Survival of the different strains under conditions of oxidative stress was tested in vitro using H2O2 as a stressor. Under high oxidative stress conditions (3 mM H2O2), the marS deletion strain showed significantly increased survival compared with that of the complementation strain (Fig. 8D). These data correspond to the situation in the kidneys of infected mice (Fig. 8A,B and C). Taken together, high oxidative stress in the host kidney correlated with a lower bacterial load. Under these conditions, bacterial DNA damage was reduced in ΔmarS compared with that in WT and survival of the deletion mutant was facilitated.
Discussion
In this study, we provide data regarding the role of the sRNA MarS in GAS M49 591 in the expression of virulence genes. GAS adheres to human tissue during colonization. Additionally, internalization by host cells has been discussed as a cause of recurrent disease, bacterial persistence in the host, and therapeutic failure of penicillin treatment35,36,37,38. Deletion of marS in GAS M49 591 resulted in a reduced adherence to human keratinocytes and a greater susceptibility to phagocytosis. The M protein supports evasion of phagocytosis25,26,39,40 and is involved in adherence and internalization processes37,41,42. Expression of emm, which encodes the antiphagocytic M protein, was dramatically reduced in ∆marS, explaining the phagocytosis and the adherence phenotype of the deletion strain. Activation of emm expression is controlled by Mga. The mga mRNA, which was one of the MarS targets predicted by IntaRNA was also decreased in the deletion strain. In the case of a direct interaction of MarS with the predicted binding site located at the 5′-end of the mga transcript, translation may be diminished in the deletion strain. In turn, decreased protein levels of Mga would lead to hampered stimulation of mga transcription by Mga. The expression of mga is positively autoregulated43. A small amount of mga transcript in ∆marS is consistent with the down-regulation of several genes that are known to belong to the Mga regulon33, including sclA and sof. A low abundance of the collagen-like surface proteins A and B, and C5a peptidase was observed in the proteome of ∆marS. Expression of the corresponding genes sclA, sclB, and scpA is known to be transcriptionally controlled by Mga44,45,46. We conclude that an influence of MarS on mga expression leads to down-regulation of mga in the deletion strain and, consequently, a down-regulation of Mga-activated genes. Direct binding of MarS to the predicted mga mRNA binding site was supported by EMSAs. The marS gene is conserved throughout GAS, and the binding site in the 5′ UTR of mga is conserved in several GAS emm types as determined by BLAST23 analysis. Amongst others, these include emm18, emm28, emm59, and emm83, which are responsible for diseases as diverse as acute rheumatic fever, puerperal sepsis, severe invasive disease, and skin tissue infections47,48,49,50. Binding of sRNAs to their target mRNAs is a typical characteristic of trans-acting sRNAs in many bacteria. Recently, direct sRNA-mRNA binding has also been observed in GAS. The interaction of FasX with its targets mRNAs prtF1 and prtF2 and cpa could be observed in vitro by gel shift assays17,18. FasX mediated regulation of pilus genes occurred in a serotype-specific manner16. Accordingly, target prediction in different GAS genomes in combination with in vitro binding studies might lead to the discovery of an emm-type specific target spectrum of MarS.
Depending on the GAS serotype, the infection model used, and the nature of the mutation, virulence of surface protein-deficient GAS strains in mice is affected differently. In a recent study, a commonly occurring single-nucleotide polymorphism (SNP) in GAS M59 increased expression of mga and 54 other genes, leading to significantly larger skin lesions in mice51. Decreased Mga activity or inactivation of mga or emm, respectively, led to attenuated virulence of GAS in mouse models for skin infection52,53,54. While fibronectin binding promoted bacterial adherence, dissemination to the spleen of infected mice was less efficient in GAS expressing fibronectin-binding protein F1 in comparison to bacteria lacking this protein55. Disruption of pilus assembly by sortase deletion rendered the GAS serotype M49 significantly more aggressive in a dermonecrotic mouse infection model56. Taken together, the down-regulation of surface-bound virulence factors leads to hampered adherence. Under these circumstances, in systemic infection models, bacterial dissemination is promoted. In our model, deletion of marS led to down-regulation of several surface proteins, including the M protein and the fibronectin-binding proteins SfbX49 and Sof. Consequently, the ability to adhere to keratinocytes was diminished, while dissemination in a sepsis mouse model was increased.
One prerequisite for successful infection is the ability of the pathogen to withstand the oxidative stress conditions generated by the host at the site of infection. GAS employs a variety of resistance mechanisms towards ROS, including physical barriers, enzymatic reactions, and metal homeostasis57. Bacterial DNA damage in ∆marS was decreased compared with that in WT under high oxidative stress conditions in the kidney, indicating that MarS influences the expression of genes involved in the oxidative stress response; however, the regulatory target remains unknown. In this context, a lack of MarS was advantageous for GAS M49 591-survival in the host.
In the proteomes of ΔmarS and in ΔmarS::marS, the abundance of the cysteine proteinase SpeB was significantly reduced compared with that in WT. SpeB production is regulated by the CovR/S two-component system and plays a specific role in invasive disease. Comparative genomics and transcriptomics revealed that invasive GAS M1 strains exhibit a SpeB switch caused by CovR/S mutations, leading to the increased expression of several virulence factor genes, including ska, slo, sda1, sic, and scpA, and to decreased SpeB abundance58,59. SpeB production is also stimulated by Mga in GAS M49 591, but there is no direct binding of the speB promoter by Mga46. The down-regulation of SpeB in ∆marS could be caused by decreased levels of Mga in this strain. However, the phenotype was not complemented by ectopic marS expression from a plasmid, indicating a more complex situation.
One of the putative targets identified by the IntaRNA algorithm was hasB, encoding the UDP-glucose 6-dehydrogenase, which is part of the capsule synthesis operon in GAS. There were no significant differences in hyaluronic acid content between WT and ΔmarS, whereas ΔmarS::marS produced significantly more capsule in comparison to the WT strain. Although the hyaluronic acid capsule is known to impact resilience to neutrophils25,26, differential capsule production was not observed in the deletion mutant and did not lead to decreased survival in the phagocytosis assay. The capsule is also known to influence the adherence of GAS to human keratinocytes42,60. In our model, ∆marS could not bind as efficiently as WT to HaCaT cells. ΔmarS::marS was able to restore the WT phenotype, but the high hyaluronic acid content of the strain did not lead to significantly increased adherence. Therefore, hyaluronic acid does not seem to play a major role as an adhesin in this serotype. GAS M49 591 naturally produces small amounts of hyaluronic acid in comparison to other serotypes. Consequently, we observed a more pronounced regulatory effect of MarS on capsule production in GAS M18 MGAS8232.
Together, MarS modulates the expression of virulence factor genes belonging to the Mga regulon and influences hyaluronic acid production in GAS, thereby promoting virulence. While FasX is a negative regulator of pili and the fibronectin-binding proteins PrtF1 and PrtF2, it upregulates the expression of streptokinase, thereby functioning as a switch from colonization to dissemination17,18. In contrast, MarS promotes adhesion by enhancing the expression of several extracellular matrix-binding surface proteins and stimulating capsule production while suppressing bacterial dissemination. We propose that MarS is involved in GAS colonization during the early stages of infection.
Methods
Bacterial strains and culture conditions
The GAS serotype M49 strain 591 was kindly provided by R. Lütticken (Aachen, Germany). The GAS serotype M18 strain MGAS8232 was obtained from the Centre of Epidemiology and Microbiology, National Institute of Public Health, Prague, Czech Republic. All GAS strains were cultured in chemically defined medium (CDM)61 or Todd-Hewitt broth (Thermo Fisher Scientific, Darmstadt, Germany) supplemented with 0.5% yeast extract (Thermo Fisher Scientific, Darmstadt, Germany) (THY), as indicated, at 37 °C with a 5% CO2/20% O2 atmosphere. Escherichia coli strain DH5α (Gibco BRL, Eggenstein, Germany) was used as a host for the construction, proliferation, and storage of recombinant plasmids. All E. coli strains were cultured in Lennox L Broth Base (Thermo Fisher Scientific, Darmstadt, Germany). For selection, antibiotics were added at the appropriate concentrations.
Construction of recombinant GAS strains
For the construction of an isogenic marS deletion mutant of GAS M49 591 (ΔmarS) and GAS M18 MGAS8232 (GAS M18 MGAS8232 ΔmarS), marS was exchanged for a spectinomycin resistance cassette by homologous recombination62. To supply sequence to mediate homologous recombination, an upstream 800 bp flanking region 1 fragment and a downstream 931 bp flanking region 2 fragment were amplified by PCR using chromosomal DNA from the parental strain as a template. All primers used for the generation of the respective fragments are listed in Supplementary Table S1. PCR products were sequentially cloned into the MCS of pUC18Erm163. Between the flanking regions, a spectinomycin resistance cassette from pFW562 was cloned into the BamHI site. The resulting suicide plasmid was verified by classical Sanger sequencing (GATC Biotech AG, Konstanz, Germany) and was used to transform GAS strains M49 591 or M18 MGAS8232. Deletion of marS was confirmed by sequencing. Therefore, a PCR product of the genomic region was analysed by classical Sanger sequencing (GATC Biotech AG, Konstanz, Germany). Loss of MarS was determined by RT-qPCR. For construction of a complementation strain (ΔmarS::marS), a fragment including the endogenous promotor and terminator regions was amplified by PCR and cloned into the SalI/BamHI sites of the shuttle vector pAT1964. The resulting vector was verified by sequencing and used for transformation of ΔmarS. The absence of spurious mutations in the recombinant strains was confirmed by MiSeq whole genome sequencing. The corresponding data were submitted to the European Nucleotide Archive (ENA/SRA) (Accession number: PRJEB18537).
Assays to assess the ability of the bacteria to survive in blood and plasma
The ability of the bacteria to survive in blood (short: blood survival assay) was assessed as described by Nakata et al.56. Briefly, overnight cultures of the GAS parental strain and isogenic mutants were inoculated into fresh medium and grown to the exponential growth phase. The cultures were centrifuged, washed and suspended in phosphate-buffered saline (PBS). Next, 20 µl of each respective cell suspension was used to inoculate 480 µl heparinized human blood. Blood was obtained from at least three individual volunteers. The samples were incubated for 3 h at 37 °C under rotation. CFUs of the samples were determined following serial dilution and plating on THY agar plates and compared to the CFUs of the respective inoculate. The resulting multiplication factor (MF) was used to compare strains. The data were normalized by setting the MF of the WT to 100%. The ability of the bacteria to survive in plasma (short: plasma survival assay) was assessed accordingly using human plasma as the medium.
Quantitative phagocytosis assay
Human neutrophils were isolated from human blood using PolymorphPrep™ (PROGEN Biotechnik GmbH, Heidelberg) according to the instructions of the manufacturer. The neutrophils were suspended in RPMI 1640 (Invitrogen, Thermo Fisher Scientific, Darmstadt, Germany). Bacteria were grown over night and washed with PBS. For opsonization 107 CFU/ml were incubated for 20 min with 10% human serum at room temperature. The opsonized bacteria were incubated with 107 human neutrophils/ml (1:1) and 5% serum for another 30 min at 37 °C. As a reference, a sample of the opsonized bacteria was incubated without neutrophils. To determine the survival rate, the samples were centrifuged and the pellets lysed in sterile distilled water. The counts of viable GAS were determined following serial dilution and plating on THY agar. To determine the proportion of extracellular bacteria, the samples were centrifuged for 5 min at 100 g for separation. The supernatant was collected, centrifuged at 13.000 g, and the bacterial pellet was dissolved in PBS.
Quantification of hyaluronic acid
The amount of cell-associated hyaluronic acid produced by GAS was determined by the release of capsule from cells in the exponential growth phase and subsequent measurement of the hyaluronic acid content using Stains-All (Sigma) as described previously37. The absorbance at 640 nm was compared to a standard curve prepared with known concentrations of hyaluronic acid. The amount of hyaluronic acid in the samples was calculated in fg/CFU. The data are expressed relative to the content of hyaluronic acid in the respective WT strain.
Adherence and internalization assay
Bacterial adherence to and internalization into the human keratinocyte cell line HaCaT (DKFZ, Heidelberg, Germany) was quantified employing an infection assay65. In brief, 24-well-plates were inoculated with 2.5 × 105 HaCaT cells per well in DMEM (Invitrogen, Thermo Fisher Scientific, Darmstadt, Germany) without antibiotics. Growth was allowed until confluence. Keratinocytes were washed with DMEM and infected separately with GAS strains of interest in DMEM at a multiplicity of infection (MOI) of 1:10. After 2 h incubation at 37 °C in a 5% CO2 atmosphere, the keratinocytes were washed extensively with PBS. To detach the keratinocytes, trypsin/EDTA (Invitrogen, Thermo Fisher Scientific, Darmstadt, Germany) was added and the keratinocytes were lysed in sterile distilled water. CFU from GAS attached to and internalized into HaCaT keratinocytes were determined following serial dilution in PBS and plating on THY agar.
Electrophoretic mobility shift assay (EMSA)
RNA:RNA EMSAs were performed as described by Danger et al.18. Briefly, RNA for RNA:RNA gel shift assays was prepared by in vitro transcription of the T7 promoter sequence containing PCR products using T7 polymerase. All primers used for the generation of the respective fragments are listed in Supplementary Table S1. Chromosomal DNA of GAS M49 591 served as the template for the mga 5′ region and the marS fragments and pAT19_ marS 88-CC-89/88-GG-89 served as the template for the mismatch marS fragment. In vitro transcription reactions were performed using the MEGAshortscript kit (Thermo Fisher Scientific, Darmstadt, Germany) according to the instructions of the manufacturer. Template DNA was removed using TURBO DNase (Thermo Fisher Scientific, Darmstadt, Germany). The RNA was purified using the RNA Clean and Concentrator-25 kit (Zymo Research Europe, Freiburg, Germany). For probe labelling, mga mRNA was biotin-labelled using the Pierce RNA 3′ end biotinylation kit (Thermo Fisher Scientific, Darmstadt, Germany). Probes were purified using the RNA Clean & Concentrator-5 kit (Zymo Research Europe, Freiburg, Germany). All RNAs were quantified using the Qubit 3.0 Fluorometer (Thermo Fisher Scientific, Darmstadt, Germany) and their quality was evaluated using the Agilent Bioanalyzer 2100 system. Labelled mga RNA (12 nM) was incubated in the presence or absence of MarS RNA (0, 10, 100, 1000 nM), mmMarS (1000 nM), unlabelled mga RNA (10, 100, 1000 nM) or unlabeled yeast tRNA (1000 nM). EMSA reactions (10 µl) contained 1 µl tRNA (10 µg/µl stock) and 1 µl of structure buffer (10 x stock; provided with the Lightshift RNA EMSA kit, Thermo Fisher Scientific, Darmstadt, Germany). Reactions were heated to 56 °C for 5 min before cooling to 37 °C for 30 min to allow refolding. REMSA loading buffer (Lightshift RNA EMSA kit, Thermo Fisher Scientific, Darmstadt, Germany) was added to each sample. The samples were separated on a 5% TBE mini-gel in 0.5 × TBE buffer, transferred by semi-dry blotting to a positively charged nylon membrane, and UV-crosslinked. The membrane was then blocked for one hour at RT (Odyssey Blocking Buffer, Li-Cor, diluted 1:3 in PBS), incubated with Streptavidin IRDye (Li-COR) at room temperature for 20 min in the dark, washed 3 x (PBST, 1% SDS), and the labeled RNA was detected using a Li-Cor Odyssey system. The membranes were rinsed and stored in PBS.
Transcript stability determination
GAS strains were grown to the transitional growth phase in THY (OD600 of 0.8) before the addition of rifampicin (to 1 mg/ ml) to inhibit RNA synthesis. Following the addition of rifampicin, 10 ml samples were recovered after 0, 1, 2, 3, 5, 10, and 15 min, as indicated. Samples were pelleted by centrifugation and quickly frozen in liquid nitrogen. Total RNA was extracted as described below.
Reverse transcription followed by quantitative PCR (RT-qPCR)
GAS strains were grown to the transitional growth phase in THY (OD600 of 0.8). Bacterial cells were either pelleted immediately and quickly frozen in liquid nitrogen or exposed to human blood for one hour prior to sample preparation. Total RNA from GAS strains was extracted according to the protocol supplied with the Direct-zolTMRNA MiniPrep Kit (Zymo Research, Irvine). After extraction, RNA was treated with acid phenol:chloroform:isoamyl alcohol (125:24:1), pH 4.5 (Thermo Fisher Scientific, Darmstadt, Germany), and TURBOTMDNAse (Thermo Fisher Scientific, Darmstadt, Germany) according to the manufacturer’s instructions. cDNA synthesis was performed using the Superscript first-strand synthesis system for RT-PCR (Invitrogen, Thermo Fisher Scientific, Darmstadt, Germany). Quantitative PCR amplification was performed with SYBR green (Thermo Fisher Scientific, Darmstadt, Germany) using the ViiA™ 7 Real-Time PCR System (Applied Biosystems, Darmstadt, Germany). The 5 S rRNA gene and the DNA gyrase subunit A gene (gyrA) served as housekeeping genes. Relative expression was calculated employing the 2−ΔΔct method66. All primers used for RT-qPCR are listed in Supplementary Table S1.
Northern blot analyses
Total RNA was isolated from GAS strains grown to the transitional growth phase in THY (OD600 of 0.8) as described above. RNA samples (10 μg) were loaded onto an 8% TBE-Urea polyacrylamide gel and separated by electrophoresis. Size standards (Ultra Low Range Ladder, Fermentas) were loaded on the same gel. RNA was electroblotted onto positively charged nylon membranes (Ambion) and UV cross-linked. Templates for the probes were generated by PCR with the same primers that were used for the PCR reaction in the RT-qPCR experiments. To the 5′ end of the reverse primers was added the T7 promoter sequence (CTTAATACGACTCACTATAGGG) for in vitro transcription (MAXIscript™ T7 Transcription Kit, Ambion). Probes were labelled with biotin prior to hybridization (Brightstar Psoralen-Biotin Labeling kit, Ambion). Membranes were hybridized overnight with a RNA probe complementary to MarS or 5 S RNA, as indicated. A BrightStar BioDetect Kit (Ambion) was used for detection, and autoradiography films were exposed to the luminescent blots.
Extract preparation for proteome analyses
Bacteria were grown in THY and samples were collected at different time points during growth. Crude extracts were prepared in a precellys 24 homogenizer (peqLab Biotechnologie GmbH, Erlangen, Germany) and divided into cytoplasm-depleted and cytoplasmic fractions by centrifugation at 13000 g. Three biological replicates were performed.
Proteome analyses
Mass spectrometry was performed on a Synapt G2-S mass spectrometer coupled to a nanoAcquity UPLC system (Waters, Manchester, UK). Peptides of the tryptic digests were separated by reversed-phase UPLC and analysed in data-independent mode (HDMSE). Label-free protein quantification and expression analysis were performed using Progenesis QI for Proteomics (Nonlinear Dynamics, Newcastle upon Tyne, UK). A detailed description of the experimental procedures is provided as supporting information (Supplementary Methods S1).
Murine infection model
Naïve, inbred, 8-week-old female BALB/c mice were purchased from Charles River Laboratories (Sulzfeld, Germany). Mice were inoculated intraperitoneally with 8 × 107 CFU of GAS strains, as indicated, in 0.2 ml PBS utilizing a BD Microlance 27 G 3/4” (Becton Dickinson GmbH, Heidelberg, Germany). Mock infection was performed with 0.2 ml PBS. As a vector control mice were infected with GAS M49 591 carrying pAT18/GFP. Twenty-four h post-infection, the mice were sacrificed using a ketamine/xylazine combination. Bacterial dissemination was investigated by determination of bacterial loads in different organs67. All the experimental protocols were approved by a licensing committee as specified in the ethics statement.
Bacterial oxidative stress resistance
GAS strains were grown in THY to the early exponential growth phase. H2O2 (Roth, Karlsruhe, Germany) was added as indicated. Following incubation for 2 h at 37 °C, cells were transferred to ice, harvested, washed twice with PBS and plated on THY agar for CFU determination.
DNA damage detection
Total DNA from mouse tissues was isolated using the DNeasy Blood and Tissue Kit (Qiagen, Hilden, Germany) according to the manufacturer’s instructions. DNA damage detection was performed as described elsewhere34. In brief, DNA quantity and purity were determined by spectrophotometric analysis. DNA lesion rates were determined by sequence-specific qPCR of mouse mitochondrial DNA (mmtDNA) and bacterial DNA, respectively. Amplification of a long (mmtDNA: 618 bp, gyrA: 775 bp) and a short (mmtDNA: 87 bp, gyrA: 85 bp) fragment was performed relative to DNA isolated from untreated cells. The small amplicon served as an undamaged DNA reference and allowed for DNA concentration normalization. PCR was performed with SYBR green (Thermo Fisher Scientific, Darmstadt, Germany) using a Light Cycler® 480 Instrument (Roche Diagnostics, Mannheim, Germany). All primers used for qPCR are listed in Supplementary Table S1. DNA was isolated from at least four animals, and qPCR reactions were performed in triplicates.
Statistical Analyses
All experiments were performed at least three times or as indicated by the sample size (n). Statistical significance was determined for normalized data using the Wilcoxon signed-rank test. RNA stability tests were performed in three biological replicates; thus, the Student’s t-test was used to calculate statistical significance. For all other experiments, the test used to determine statistical significance is indicated in the respective figure legend.
Ethics statement
The protocol for the collection of human blood for the blood survival assay was approved by the Ethikkommission an der Medizinischen Fakultät der Universität Rostock (ethics committee vote: A 2014-0131). The experiments were conducted in accordance with the ICH-GCP guidelines. Informed consent was obtained from all subjects. The protocol for the murine infection model was approved by the Landesamt für Landwirtschaft, Lebensmittelsicherheit und Fischerei M-V (Permit Number: 7221.3-1.1-090/12). Mice were sacrificed using a ketamine/xylazine combination. Animal experiments were performed in strict accordance with the German regulations of the Society for Laboratory Animal Science (GV-SOLAS) and the European Health Law of the Federation of Laboratory Animal Science Associations (FELASA).
Data availability
The whole genome sequencing datasets generated during the current study are available in the European Nucleotide Archive (ENA/SRA) repository (Accession number: PRJEB18537). The proteome data generated during this study are included in this published article (and its Supplementary Information files). All additional datasets generated during or analysed during the current study are available from the corresponding author upon reasonable request.
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Acknowledgements
We thank Brigitte Vollmar and the Core Facility “Zentrale Versuchstierhaltung“ in the Rudolf-Zenker-Institut für Experimentelle Chirurgie, Universitätsmedizin Rostock, for laboratory animal care. The BMBF provided funding for Bernd Kreikemeyer in the framework of the ERA-Net PathoGenoMics 2 programme (FKZ 0315437B). The work of Nadja Patenge was supported by the University Medicine Rostock (Forun 889012). Sonja Oehmcke-Hecht was supported by a grant from the Deutsche Forschungsgemeinschaft (OE 547/2-1). Torsten Hain was supported by LOEWE Medical RNomics and the German Centre for Infection Research, Justus-Liebig University Giessen. The Synapt G2-S mass spectrometer was acquired with funds from “Europäischer Fonds für regionale Entwicklung“ (EFRE), # 2007DE161PO003, awarded to the University Medicine Rostock.
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Conception and design for this study: N.P., R.P., P.W., S.M., and B.K. Acquisition, analysis, and interpretation of the data: R.P., P.W., S.M., J.N., A.W.-K., F.H., M.W., A.K., O.S., S.O.-H., T.H. and N.P. Drafting or revising the article: N.P., R.P., P.W., S.M., and B.K. All authors read and approved the final manuscript.
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Pappesch, R., Warnke, P., Mikkat, S. et al. The Regulatory Small RNA MarS Supports Virulence of Streptococcus pyogenes . Sci Rep 7, 12241 (2017). https://doi.org/10.1038/s41598-017-12507-z
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DOI: https://doi.org/10.1038/s41598-017-12507-z
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