Aerotolerance and Peroxide Resistance in Peroxidase and PerR Mutants of Streptococcus pyogenes

doi:10.1128/JB.182.19.5290-5299.2000

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Journal of Bacteriology, October 2000, p. 5290-5299, Vol. 182, No. 19
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Aerotolerance and Peroxide Resistance in Peroxidase and PerR Mutants of Streptococcus pyogenes

Katherine Y. King, Joshua A. Horenstein, and Michael G. Caparon^*

Department of Molecular Microbiology, Washington University School of Medicine, St. Louis, Missouri 63110-1093

Received 25 October 1999/Accepted 6 July 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Survival in aerobic conditions is critical to the pathogenicity of many bacteria. To investigate the means of aerotoleranceand resistance to oxidative stress in the catalase-negative organismStreptococcus pyogenes, we used a genomics-based approach to identifyand inactivate homologues of two peroxidase genes, encoding alkylhydroperoxidase (ahpC) and glutathione peroxidase (gpoA). Singleand double mutants survived as well as the wild type under aerobicconditions. However, they were more susceptible than the wildtype to growth suppression by paraquat and cumene hydroperoxide.In addition, we show that S. pyogenes demonstrates an inducibleperoxide resistance response when treated with sublethal dosesof peroxide. This resistance response was intact in ahpC and gpoAmutants but not in mutants lacking PerR, a repressor of severalgenes including ahpC and catalase (katA) in Bacillus subtilis.Because our data indicate that these peroxidase genes are notessential for aerotolerance or induced resistance to peroxidestress in S. pyogenes, genes for a novel mechanism of managingperoxide stress may be regulated by PerR instreptococci.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Adaptation to an aerobic environment provides organisms with a wider selection of ecological niches for survival. The majorcost associated with this evolutionary gain is constant exposureto the deleterious effects of oxygen, particularly the partiallyreduced forms of oxygen that include peroxide, superoxide, andhydroxyl radicals (23). In response to this toxic exposure,aerobic organisms have evolved powerful strategies to defend themselvesagainst the damaging effects ofoxygen.

The group of organisms collectively known as the lactic acid bacteria provides a useful example of adaptation to the aerobicenvironment. Unlike organisms that have evolved a system of oxidativephosphorylation, these bacteria have an exclusively fermentativemetabolism, and they lack many of the well-characterized enzymesthought to be essential for aerobic survival (13). Nevertheless,most lactic acid bacteria are aerotolerant to some degree andthus are considered facultative anaerobes. Surprisingly, growthis unaffected or even enhanced by exposure to oxygen for somespecies (38).

Recent investigations have suggested that interaction with oxygen plays an important role in the pathogenesis of infectionscaused by the lactic acid bacterium Streptococcus pyogenes. Thisbacterium is an important human pathogen that is responsible forvarious diseases, including soft tissue infections that rangefrom minor and self-limiting (pharyngitis, impetigo) to severelydestructive and life-threatening (necrotizing fasciitis). Toxigenicinfections (toxic shock syndrome) and several autoimmune diseases(rheumatic fever, acute postinfectious glomerulonephritis) arealso associated with infection by S. pyogenes. Adhesion to hosttissues is likely to be an early event in pathogenesis for allof these diseases. Expression of a major adhesin, the fibronectin-bindingprotein known as protein F or Sfb, is environmentally regulated,being preferentially expressed in aerobic environments (51).Regulation occurs at the level of transcription and is apparentlylinked to a pathway that senses oxidative stress (22). Theseobservations suggest that S. pyogenes encounters and reacts toan aerobic environment duringinfection.

Consistent with an at least partially aerobic lifestyle, most isolates of S. pyogenes are highly aerotolerant, and growthyields can actually be increased under aerobic conditions whengrown on certain substrates (21). To thrive in an aerobic environment,it is likely that S. pyogenes must possess mechanisms for defenseagainst reactive oxygen species. A critical issue concerns defenseagainst hydrogen peroxide (H₂O₂), a highly reactive molecule thatcan readily diffuse across cellular membranes and oxidativelydamage a number of vital cellular components, including membranelipids, enzymes, and DNA (39, 44). Not only may S. pyogenesencounter peroxide during the infection of tissue but, like manyother lactic acid bacteria, S. pyogenes also has the capacityto produce large amounts of peroxide endogenously when it is growingunder aerobic conditions (21). A large body of evidence collectedfrom analysis of multiple bacterial species has implicated catalase,a heme-containing peroxidase, as the major factor responsiblefor defense against peroxide (19). The importance of catalaseis further emphasized by the fact that most facultative and aerobicbacteria contain multiple catalases (14). However, as is characteristicof lactic acid bacteria, S. pyogenes does not synthesize hemeand lacks catalase (13). The specific mechanisms by which S.pyogenes adapts to peroxide stress areunknown.

In this study, we have examined the adaptive response of S. pyogenes to peroxide stress and the potential contribution ofalternative peroxidases to this response. Using a genomics-basedapproach, we found that S. pyogenes contains homologues of twoperoxidases that have been characterized in other species. Constructionand analysis of several mutants revealed that these peroxidasescontribute to defense against high-level oxidative stress. Incontrast, the inactivation of these genes neither impairs growthunder aerobic conditions nor hinders the ability of S. pyogenesto mount an adaptive response against peroxide. Interestingly,this adaptive response was constitutively induced in mutants lackingPerR, a negative regulator of several genes, including ahpC andcatalase (katA) in Bacillus subtilis. However, because these lattertwo genes do not appear to be essential to the S. pyogenes adaptiveresponse, PerR may control expression of genes responsible fora potentially novel strategy for adaptation to aerobic growthenvironments in S. pyogenes.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains, media, and growth conditions. The host for molecular cloning experiments was Escherichia coli DH5 $alpha$ . For peroxide resistance experiments involving E. coli,strain CH734 was used. For probing of $sigma$ ^B genes by PCR, the following bacterial strains were used: Staphylococcusaureus Newman (16), Listeria monocytogenes 104035 (45), andB. subtilis Marburg 168 (34). Luria-Bertani broth (48) ortryptone agar (137 mM NaCl, 1% tryptone [wt/vol], 0.1% yeast extract[wt/vol], and 1.4% agar) were used to culture E. coli. Strainsof S. pyogenes were grown in Todd-Hewitt medium (BBL) supplementedwith 0.2% yeast extract (THY medium) at 37°C. To prepare solidmedium for S. pyogenes, Bacto Agar (Difco) was added to THY mediumto a final concentration of 1.4%. Various atmospheres for culturesof S. pyogenes were created using conditions established in priorinvestigations (22). Briefly, for aerobic cultures, streptococciwere grown on solid medium in ambient air (20% O₂, 0.03% CO₂)or in liquid medium in a 125-ml Erlenmeyer flask filled to 8%of its total volume on an orbital shaker rotating at 225 rpm.For near-anaerobic cultures, streptococci were grown staticallyin 10 ml of liquid medium in a sealed 15-ml culture tube. Foranaerobic cultures, streptococci were incubated on solid mediain a sealed jar with a commercial gas generator (GasPak catalogueno. 70304; BBL), or in a 10-ml volume of liquid media in a sealed15-ml culture tube with a commercial additive to produce anaerobicconditions (Oxyrase). When appropriate, the following concentrationsof antibiotics were used: 50 µg of kanamycin, 750 µg of erythromycin,3 µg of chloramphenicol, and 100 µg of ampicillin per ml for E.coli cultures and 500 µg of kanamycin, 3 µg of chloramphenicol,and 1 µg of erythromycin per ml for S. pyogenescultures.

Computational analyses. Genome sequence databases for S. pyogenes at the University of Oklahoma (http://www.genome.ou.edu/strep.html) and the SangerCenter (http://www.sanger.ac.uk/Projects/S_pyogenes) were searchedfor homologues to a set of known bacterial peroxidases. The sequencesused as queries in TBlastN (1) searches included: thiol peroxidase(GenBank accession no. AAC74406), Mn²⁺-pseudocatalase (no. BAA13239), the catalase of the heme-scavenginglactic acid bacteria Lactobacillus sake (no. AAC19139),NADH peroxidase (no. 1942624), alkyl hydroperoxide reductase (no.BAA25695), and glutathione peroxidase (no. AJ000109).The S. aureus $sigma$ ^B gene (no. CAA68932) was used to computationally searchfor a $sigma$ ^B homologue. The PerR gene (no. Z99108, originally named ygaG;see reference 4) was used to identify its homologue in S. pyogenes.

DNA techniques. Plasmid DNA was isolated by standard techniques and transformed in E. coli as described by Kushner (37). Transformationof S. pyogenes was performed by electroporation as previouslydescribed (6). Restriction endonucleases, ligases, and polymeraseswere used according to the manufacturers' recommendations. ChromosomalDNA was purified from S. pyogenes as previously described (6).Hybridization analysis was done according to the method of Southern(50), and probes of appropriate sequences were labeled with³²P by a random priming method (Rediprime; Amersham). For amplificationof $sigma$ ^B from purified chromosome of various bacteria, primers based onhighly conserved regions of $sigma$ ^B were used: sigb5 (CTCCG TGATA AAACA TGGAG CGTTC ATG) and sigb3(CGAGA GACAT GCATT TGTGA TATACCGAG).

Deletion of ahpC. An in-frame deletion in the gene encoding the peroxidase subunit (ahpC) of alkyl hydroperoxide reductase was constructed asfollows. Primers ahp5' (AAAAG GGGTA CCACT ATATG TCTC) and ahp3'(GCCAT AGCTT GGATC CTAAA ATTTA) were used to amplify a 604-bpfragment containing the entire ahpC open reading frame (see Results)from S. pyogenes strain JRS4. The PCR product was digested withthe restriction enzymes KpnI and BamHI (sites in primers as underlinedabove) and inserted between the corresponding restriction sitesof pUC18 (Boehringer Mannheim) to create pJH2. Digestion of pJH2with BstEII, followed by treatment with ligase, deleted a regioninternal to ahpC between nucleotides 155 and 292 while conservingthe correct reading frame (see Fig. 1). The resulting allele (ahpC_155-292)was inserted between the SmaI and PstI sites of the E. coli-streptococcalshuttle vector pJRS233 (42) to create pJH4. This plasmid wasused to replace the wild-type ahpC allele in several S. pyogenesstrains using a previously described method (47). The chromosomalstructure of mutant alleles was confirmed by PCR and hybridizationanalysis (50).

Deletion of gpoA. An in-frame deletion in the gene encoding GpoA was constructed using an approach similar to one that has been previously described(47). A 579-bp region corresponding to the entire gpoA codingregion was amplified from HSC5 chromosomal DNA by PCR using primers:glu5' (CCGTT GACCA AATTA TCAGT TACAC CGAGG ATCCG TCACA TGCC) andglu3' (GAAGT TTTTA ATTAG TAACT ATAAT ATAAA ATAGA ATTCG CACGC C).This PCR product was inserted into a commercial vector (pCR2.1;Invitrogen) by a TA-tail technique to make pJH5 (31). Inside-outPCR was performed on pJH5 using primers gluIFD5' (GTCAA CTAGTGAGAT GTGTC GACCG TCCTG AGCCT TAACC G) and gluIFD3' (CCTTG CAACCAATTT TTAAA TCAAG GTCGA CGAGA TGCTG AGGAG). The PCR product wasdigested with SalI (sites in each primer are underlined) and subjectedto ligation. The resulting gpoA allele contains an in-frame deletionspanning residues 42 to 212 (gpoA_42-212). This allelewas then inserted between the XhoI and HindIII sites of the E.coli-streptococcal shuttle vector pJRS233, which was used to replacethe mutant allele with the wild-type allele in two streptococcalstrains as described above. The mutant alleles and chromosomalstructures were confirmed by PCR and hybridizationanalysis.

For construction of an ahpC-gpoA double mutant, an internal region of the gpoA gene was amplified by PCR using the primers5Gpo (GTCAC ATGCC GAATT CCTAT GATTT TACGG) and 3Gpo (CCATT CACTTTGAAT TCTGC AAAGC GAGGG). This product was digested with the restrictionenzyme EcoRI (sites in each primer are underlined) and insertedinto the EcoRI site of the integrational vector pCIV2 (41) toproduce pKK15. Introduction of pKK15 into ahpC mutant HAHP resultedin the insertional inactivation of gpoA and generated the doublemutant HAG. An ahpC-gpoA double mutant was constructed in a JRS4background by sequential replacement of the ahpC and gpoA alleleswith their mutant counterparts as described above (see Table 1).

Disruption of perR. An in-frame deletion in the gene encoding PerR was constructed using an approach similar to that used to disrupt gpoA. An880-bp region corresponding to the entire perR coding region wasamplified from HSC5 chromosomal DNA by PCR using primers: 5PerIXhoI'(CGTTT CAAAA TCCCT CGAGG ATGTC CTAAA AGC) and 3PerSacI' (GGGATACGCG TGAGC TCATA ACCTG TTTG). This PCR product was digested usingthe restriction enzymes XhoI and SacI (sites in primers underlined)and inserted into the corresponding restriction sites in a commercialvector (pCR2.1; Invitrogen) to produce pKK12. Inside-out PCR wasperformed on pKK12 using primers 5Per2SalI' (GAGCC TTTGC CACAG TCGACAATAA TTTG) and 3Per2SalI' (GTGAA TGAAT GTCGA CAAGC TGCTA CTCC),and the product was digested with SalI (sites in each primer areunderlined) and subjected to ligation. The resulting perR allelecontains an in-frame deletion spanning residues 1 to 66 (perR_1-198),including the initial methionine residue and most of the putativeDNA-binding region of the protein. This allele was then insertedinto the HindIII site of the E. coli-streptococcal shuttle vectorpJRS233, which was used to replace the mutant allele with thewild-type allele in two streptococcal strains as described above.The mutant alleles and chromosomal structures were confirmed byPCR.

Construction of reporter plasmids. A 1.1-kb genomic fragment upstream and including the first 10 codons of ahpC were amplified by PCR using the primers 5AhpPro(CCTTG TGCCA TATGG ATCCA CTTCC TTTC) and 3AhpPro (GCTTG AGCTGAGAAT TCAGC AATTT CTTAT CC) (see Fig. 1). This region includedall of the intervening sequence between ahpC and the next upstreamand divergently transcribed open reading frame that showed homologyto a cold shock protein E gene. Similarly, the 335-bp genomicfragment upstream and including the first 35 codons of the oligoendopeptidaseF gene that immediately precedes gpoA in an apparent operon wereamplified using the primers 5GpxPro (CCTAA ATAAT CAGGA TCCGT ATTATTTTGA) and 3GpxPro2 (GAACG TTTTT TGAAT TCCAT AGTTG TCTCC TAAAC)(see Fig. 2). This region includes the intervening region betweenthe oligoendopeptidase gene and the upstream and divergently transcribedphosphoenolpyruvate carboxylase gene. The 411-bp genomic fragmentupstream of and including the first 36 codons of mrgA was amplifiedusing the primers 5MrgPro (CTCTT GACCA TTATC AGGAT CCTAA AGTAG)and 3MrgPro (GCCAC AGAGA ATTCA GCGAC AGCTT AGTTT AAAAC).This fragment encompasses the entire region between MrgA and adivergent upstream open reading frame with homology to a type4 prepilin-like peptidase gene. Each primer contained either aBamHI or EcoRI restriction site (underlined). In addition, the3' primers contained a stop codon in the relevant reading frameto prevent translational fusions with the reporter (boldface).These PCR products were inserted between the EcoRI and BamHI restrictionsites of pABG5 (24) to place the fragment upstream of phoZF,which encodes a secreted reporter with alkaline phosphatase activity(24). These plasmids were confirmed by determination of theinsert DNA sequence and are hereafter referred to as pAhpPho,pGpoPho, and pMrgPho,respectively.

Expression of ahpC and gpoA. The ahpC, gpoA, and mrgA reporter plasmids constructed in the previous section were introduced into various S. pyogenes hostsand used to assess expression in the presence or absence of inducingconcentrations of H₂O₂ (50 µM), ethanol (5%), cumene hydroperoxide(0.025%), or methyl viologen (10 mM). Activities of the variousreporters were also compared between the wild type and perR mutants.The plasmids pABG5, in which a rofA promoter controls phoZF, andpABG6, a derivative of pABG5 in which the rofA promoter has beeninactivated, were used in parallel experiments as positive andnegative controls, respectively (24). Expression was monitoredby determination of alkaline phosphatase activity in cell-freeculture supernatants as described previously (24).

Analysis of methyl viologen sensitivity. Sensitivity to the oxidative-stress-promoting compound methyl viologen (paraquat) was evaluated as follows. Methyl viologen(Sigma) was added to liquid THY medium up to a final concentrationof 10 mM. This medium was then inoculated with 5 µl of an overnightculture grown in near-anaerobic conditions. The culture densitywas determined by measuring the absorbance (optical density at600 nm [OD₆₀₀]) after static incubation for 18 h at 37°C. Thesame analysis was conducted in the presence of catalase (1 mg/ml;Sigma) or in the presence of hemoglobin (1 mg/ml; Sigma). Theactivity of superoxide dismutase in S. pyogenes was assayed aspreviously described (22).

Sensitivity to peroxides. The strain of interest was cultured under near-anaerobic conditions to mid-log phase and a 50-µl aliquot was spread evenlyover the surface of a THY agar plate. A 10-µl aliquot of variousconcentrations of hydrogen peroxide (Sigma) diluted in water orcumene hydroperoxide (Sigma) at a concentration of 20% (vol/vol[in ethanol]) was then added to a sterile 10-mm-diameter filterdisk placed at the center of each plate. After incubation at 37°Cfor 16 h under aerobic conditions, the area of the zone of inhibitionwas calculated for each mutant and compared to that of the respectivewild-typestrain.

Characterization of resistance to hydrogen peroxide challenge. The ability of various strains to survive a lethal challenge by H₂O₂, with or without prior H₂O₂ exposure, was determinedas follows: a 10-µl aliquot of an anaerobic overnight liquid culturewas used to inoculate 10 ml of medium which was then incubatedunder near-anaerobic conditions at 37°C. When the absorbance (OD₆₀₀)of this culture reached 0.040, H₂O₂ was added to a sublethal concentration(50 µM), and the incubation continued until the OD₆₀₀ reached0.070. At this time, H₂O₂ was added to a final concentration of4 mM. After an additional 3 h of incubation, the number of CFUwas determined under anaerobic conditions. The relative survivalwas calculated by the method of Rallu et al. (46) as the percentageof bacteria surviving 3 h after lethal challenge divided by thepercentage of wild-type nonpretreated bacteria surviving 3 h afterchallenge. The ability of other agents to induce resistance toH₂O₂ was assessed by substitution of the initial inducing doseof peroxide with either ethanol (5% [vol/vol]), nalidixic acid(250 µM; Sigma), or mitomycin C (200 nM; Sigma). The inducingdose used for each agent represents the highest concentrationof that agent which did not inhibit bacterial growth during anovernight incubation under near-anaerobic conditions. For comparison,the sensitivity of E. coli CH734 to H₂O₂ was determined usingthe same assay except that Luria-Bertani medium was substitutedfor THYB. The data reported represent the mean and standard errorof the mean derived from at least two independent experiments,each of which was conducted intriplicate.

In selected experiments, the viability of cultures was assessed by using a vital stain (Live/Dead Cell Viability Kit; MolecularProbes) and microscopic observation or by determining numbersof CFU following brief sonication (Branson model W-185, 22°C,microprobe at setting of 6, five bursts of 5 s each) to disruptthe streptococcal chains. However, since the differences betweenviable cells counted before or after challenge were similar tothat derived by the direct determination of CFU, neither procedurewas routinelyperformed.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Identification of peroxidases in the S. pyogenes genome. Since S. pyogenes lacks catalase, we hypothesized that it contains an alternative peroxidase. The available S. pyogenes genomeinformation was evaluated for the presence of potential homologuesto other known bacterial peroxidases (see Materials and Methods).Only three sequences in the S. pyogenes genome database showedsignificant homology to the peroxidase genes used in the searches(P < 0.05). The first sequence appeared homologous to NADH peroxidase(GenBank accession no. 1942624) of B. subtilis; however, geneticand biochemical studies have identified this gene as NADH oxidase(21). Of the other two open reading frames identified, the firstshowed homology to the peroxidase subunit of alkyl hydroperoxidereductase (ahpC) (17) (see Fig. 1). Subsequently, the readingframe downstream of this ahpC homologue was found to be similarto ahpF. In B. subtilis, these two genes encode a two-subunitprotein complex and are known to form an operon (3). The otheropen reading frame identified showed homology to the glutathioneperoxidase (gpoA) of Lactococcus lactis (see also Fig. 2). Inaddition to a high overall level of homology, each of these twoputative peroxidases contained highly conserved residues locatedin the active sites of these enzymes known to be essential fortheir respective peroxidase activities (Fig. 1 and 2).

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FIG. 1. Alkyl hydroperoxide reductase gene in S. pyogenes. The position and direction of the ahpC gene is depicted relative to its neighbors in the genome. The percent amino acid identity and similarity to the closest match found by a TBlastN search are shown. The region inserted into the reporter plasmid for expression studies is underlined. Below is a partial alignment of the S. pyogenes ahpC gene with the Salmonella enterica serovar Typhimurium homologue. Regions around the conserved cysteines (C46 and C165) are shown. The 45-amino-acid region removed by deletion is indicated by the arrows.

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FIG. 2. Glutathione peroxidase gene in S. pyogenes. The position and direction of gpoA is shown relative to its upstream neighbor. The percent amino acid identity and similarity for the closest match found in a TBlastN search are shown. The region inserted into the reporter plasmid for expression studies is underlined. Below is a partial alignment of four glutathione peroxidase genes, showing the conserved cysteine (C36), asparagine (N99), and C-terminal region (including N125). The region of the in-frame deletion is indicated by arrows. In the process of making the deletion, a proline and a glycine (underlined) were replaced by arginines.

Construction of mutants. In order to analyze the contribution of these putative peroxidases to the aerobic growth of S. pyogenes, we constructed mutantsin which these genes were inactivated. Since it was anticipatedthat these mutants may have growth defects and since the transcriptionalorganization of these loci has not been characterized, in-framedeletions were constructed to create stable nonpolar mutations.For alkyl hydroperoxide reductase, a deletion was introduced intoahpC which removed 45 amino acids from the central region of thepolypeptide that was anchored amino terminally in a highly conserveddomain immediately adjacent to the putative active site residueC46 (Fig. 1). For gpoA, a region encompassing 57 amino acid residueswas removed, including a cysteine (C36) and the highly conservedresidues surrounding it that are constituents of the active site(Fig. 2) (17). These mutations were introduced into two unrelatedstrains of S. pyogenes (JRS4 and HSC5) to construct mutants defectivein one or both of these peroxidases (Table 1).

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TABLE 1. S. pyogenes strains

Characterization of stress phenotypes. Alkyl hydroperoxide reductase catalyzes the pyridine nucleotide-dependent reduction of organic hydroperoxides and H₂O₂ (43).Recent evidence also implicates these proteins in enzymatic defenseagainst reactive nitrogen species (9). Mutants lacking functionalAhpC or AhpF in some other organisms are hypersensitive to organichydroperoxides such as cumene hydroperoxide (3). The S. pyogenesahpC mutants were examined for a similar phenotype in a disk diffusionassay which revealed an enhanced sensitivity to cumene hydroperoxide,with zones of growth inhibition approximately 130% larger thanthose of the wild type when tested over a broad range of concentrations(5 to 20% cumene hydroperoxide). Glutathione peroxidases havebeen best characterized from mammalian cells and are also thoughtto provide protection from both H₂O₂ and organic hydroperoxides(18, 49). Their function in prokaryotic cells has been lesswell studied; however, glutathione peroxidase-defective mutantsof Neisseria meningitidis are hypersensitive to oxidative stressinduced by methyl viologen (40). Similarly, gpoA mutants ofS. pyogenes demonstrated an enhanced sensitivity to methyl viologenwhich was apparent as the inability to grow in the presence ofa concentration of methyl viologen that did not affect the growthof the wild-type strain (see below). Strains with mutations inahpC also demonstrated this sensitivity (seebelow).

Growth phenotypes of peroxidase mutants. The gram-positive bacterium B. subtilis contains both a catalase and an alkyl hydroperoxide reductase (5). Mutations inthe genes encoding either peroxidase have no effect on the abilityof the organism to grow under aerobic conditions (5). However,a mutant that is simultaneously defective for both grows verypoorly aerobically (5). Since S. pyogenes is naturally catalasedeficient, it was expected that an ahpC mutant would be equivalentto the B. subtilis peroxidase double mutant and would demonstratepoor aerobic growth characteristics. However, the S. pyogenesahpC mutants did not demonstrate any observable growth restrictionswhen examined under several types of aerobic culture, includingculture on solid medium in ambient air and culture in liquid mediumin a shaking flask (data not shown). In addition, the ahpC mutantsdid not demonstrate any increased sensitivity to H₂O₂ when analyzedboth by a disk diffusion assay and by determination of MICs (datanot shown). Identical results were obtained for gpoA-deficientmutants.

Peroxidase mutants are sensitive to methyl viologen. Although the various peroxidase mutants were proficient for growth under aerobic conditions, they did demonstrate sensitivityto certain forms of extreme oxidative stress. Specifically, whencultured in the presence of a concentration of methyl viologenthat has minimal impact on the growth of the wild-type strains(10 mM) neither the ahpC- nor the gpoA-deficient mutants demonstratedany detectable growth (Fig. 3). The ahpC gpoA double mutant waseven more sensitive to methyl viologen than the single mutants,with no growth at a concentration of 1 mM (data not shown). Methylviologen acts to increase intracellular levels of superoxide (27).Since mutants expressed superoxide dismutase at levels equivalentto those for the wild-type cells (data not shown), it is unlikelythat superoxide is the source of lethal stress to the mutants.Rather, since H₂O₂ is a product of the dismutation of superoxide,high levels of superoxide could also result in increased concentrationsof H₂O₂ and, in turn, other reactive species generated from thereaction of H₂O₂ with a variety of substrates. This hypothesisis supported by the observation that the addition of catalasecould rescue the growth of the peroxidase mutants in the presenceof methyl viologen, but the same effect was not seen with theaddition of hemoglobin (Fig. 3). A small stimulation of growthabove background values in the presence of methyl viologen wasobserved when hemoglobin was added (Fig. 3), which may be dueto the weak peroxidase activity of hemoglobin (20). These dataindicate that AhpC and GpoA contribute to defense under conditionsof extreme and continuous oxidative stress and that both peroxidasegene products are required for optimal resistance.

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FIG. 3. Methyl viologen sensitivity of ahpC and gpoA mutants. Methyl viologen (MV) sensitivity of ahpC and gpoA mutants. The growth of HSC5 (wild type), HAHP ( $Delta$ AhpC), and HGLT ( $Delta$ GpoA) in the absence (no treatment) or presence of the indicated concentrations of methyl viologen are shown. Where indicated, cultures were supplemented with catalase or hemoglobin (see Materials and Methods). Growth was measured by determining the OD₆₀₀ after 18 h of incubation. A representative experiment is shown. Similar experiments were done with HAG, JRS4, and mutants derived from JRS4 (JAHP, JGLT, and JAG, see Table 1), with similar results.

AhpC and GpoA are not required for an induced resistance to peroxide. The observation that neither AhpC nor GpoA were required for normal growth under aerobic conditions suggested that S. pyogenesmay have alternative strategies for resistance to peroxide. Toexamine this question, the kinetics of interaction with peroxidewere examined in greater detail. When a culture of a wild-typestrain was challenged at mid-log phase (approximately 10⁶ CFU) with 4 mM H₂O₂ and the number of CFU was examined after2 h, it was observed that the number of viable CFU decreased ca.0.4 log. When examined at 3 h, the number of viable CFU had decreasedby >3.0 log (data not shown). These values were actually lessthan those obtained for a culture of E. coli CH734 under thesesame conditions, for which the number of CFU decreased by about2.0 log after 2 h and >4 log after 3 h (data not shown). Thesedata suggest that, under these conditions, S. pyogenes is nothypersensitive to peroxide compared to E. coli, a catalase-containingbacterium. Furthermore, when ahpC and gpoA mutants were examined,instead of demonstrating an enhanced sensitivity, they were infact more resistant to peroxide challenge, with viability decreasingby only about 1.5 log 3 h after challenge (data not shown). Asimilar phenomenon has been reported for alkyl hydroperoxide reductase-deficientmutants of B. subtilis, where it appears that inactivation ofthe ahpC results in low-level oxidative stress sufficient to inducean adaptive resistance response to peroxide (3).

These data suggest that S. pyogenes may also possess an adaptive resistance response to peroxide. To test this, growing cultureswere treated with a sublethal dose of H₂O₂ (50 µM) 1 h prior tochallenge with a lethal dose (4 mM). As before, viability wasexamined after an additional 3 h of incubation. When treated inthis fashion, wild-type strains were >100-fold more resistantto lethal peroxide challenge (Fig. 4; wild type, H₂O₂ induction).Similar to the wild type, both ahpC and gpoA mutants were protectedby pre-exposure to a sublethal concentration of H₂O₂ (Fig. 4;AHP, H₂O₂ induced; GPO, H₂O₂ induced). Bacteria containing mutations in both ahpC andgpoA were approximately 10 times more sensitive to peroxide challengethan wild-type bacteria (Fig. 4; AHPGPO, no induction). Nonetheless, the double mutants demonstrateda striking resistance response; when pretreated with sublethalperoxide, they were up to 1,000 times more resistant to lethalperoxide challenge than without pretreatment (Fig. 4; AHPGPO, H₂O₂ induced). Taken together, these data indicate that S. pyogenescan mount a vigorous adaptive response to peroxide stress andthat this response does not require the contributions of AhpCor GpoA.

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FIG. 4. Induction of resistance response by hydrogen peroxide and ethanol. Bacterial cultures were induced with a sublethal dose of hydrogen peroxide before challenge with a lethal dose. The relative survival was calculated as the percentage of CFU after lethal peroxide challenge divided by the percentage of wild-type cells surviving the same challenge (black bars). Some cultures were not induced before challenge. Other cultures were induced with agents other than hydrogen peroxide (as indicated) before lethal challenge with H₂O₂. Each bar represents the average of at least two independent experiments, each done in triplicate. Error bars represent the standard error of the mean.

As an additional test for involvement of AhpC and GpoA in inducible peroxide resistance, we studied expression of the peroxidasegenes. Reporter plasmids were constructed by inserting the genomicregions upstream of ahpC and gpoA before a promoterless alkalinephosphatase reporter. Expression of the two reporter alleles inS. pyogenes was comparable with that of the well-characterizedrofA promoter in this vector, indicating that functional promoterswere identified by this analysis. However, expression of the ahpCand gpoA reporters did not increase in wild-type cells in thepresence of inducing levels of H₂O₂ or ethanol (data not shown).In addition, alkaline phosphatase activity from both reporterswas not higher in wild-type cells that were incubated in the presenceof 10 mM methyl viologen or 0.025% cumene hydroperoxide (datanot shown). These findings lend further support to the observationthat AhpC and GpoA are not part of the adaptive response to peroxidestress.

Peroxide resistance can be induced by ethanol. Insight into the pathway which controls an adaptive response can often be gained from an examination of whether the responseis induced by a specific stress or whether other stress-promotingagents can induce the protective response against the agent ofinterest (19). The SOS response is a highly regulated responseinvolved in resistance to agents which damage DNA, including H₂O₂(56). However, treatment with two different agents known toinduce the SOS response (mitomycin C and nalidixic acid) (56)resulted in a level of killing by H₂O₂ that did not differ fromuntreated cultures (Fig. 4; compare wild type uninduced to treatmentwith nalidixic acid or mitomycin C). Similar results were obtainedin parallel experiments with the ahpC and gpoA mutants (Fig. 4).In contrast, treatment with a sublethal concentration of ethanol(5% [vol/vol]) was highly effective at inducing a protective responseto subsequent challenge with a lethal dose of peroxide in wild-typebacteria and in both peroxidase mutants (Fig. 4). In fact, underthese conditions, ethanol was a more effective inducing agentthan H₂O₂ itself (Fig. 4, wildtype).

S. pyogenes may lack $sigma$ ^B. In gram-positive bacteria, a large number of stress-induced genes are regulated by a pathway known as the general stress response(53). Since induction by ethanol is a signature of the generalstress response (52), the possibility existed that the observedadaptive response to H₂O₂ was a manifestation of this pathway.A key element in the regulation of the general stress responseis the alternative sigma factor $sigma$ ^B and its interaction with the anti-sigma factor RbsW (25, 53).This sigma factor is highly conserved among gram-positive organisms,including S. aureus, L. monocytogenes, and B. subtilis (36,53, 54). The genes encoding $sigma$ ^B in each of these three species are between 59 and 66% identicalat the amino acid level. However, when the available S. pyogenesgenome information was examined, there were no sequences withsignificant (P < 0.33) similarity to the S. aureus $sigma$ ^B gene other than the housekeeping sigma factor $sigma$ ^A. Similarly, no clear homologues to other elements of the $sigma$ ^B pathway were apparent, including RsbU and RsbW. As an alternativeapproach, primers for PCR amplification were designed based onan examination of highly conserved elements of the $sigma$ ^B gene sequence. While a PCR product of the expected size was amplifiedusing these primers from several different gram-positive organisms,no product was amplified when the chromosome of S. pyogenes strainsthat display the adaptive response was used as a template (datanot shown). These data indicate that while the adaptive responseof S. pyogenes to peroxide shares many phenotypic characteristicsof the general stress response, the $sigma$ ^B pathway is either highly divergent or may be missingaltogether.

Regulation of the inducible peroxide resistance response involves PerR. In addition to the $sigma$ ^B general stress pathway, B. subtilis also harbors a specific response to hydrogen peroxide stress. Theperoxide-sensitive PerR regulon in that species is known to takepart in the transcriptional regulation of peroxidases such ascatalase and alkyl hydroperoxidase and of protective proteinssuch as MrgA, a DNA-binding protein (4, 10). Mutational analyseshave indicated that PerR is a negative regulator of katA, ahpC,and mrgA expression in B. subtilis. Notably, mutants lacking PerRwere found to be hyper-resistant to hydrogen peroxide in a diskdiffusion assay. Examination of the genome information and otherpublished work suggests that S. pyogenes contains homologues forperR and mrgA in addition to ahpC (4). To analyze the roleof PerR, we constructed an in-frame deletion that removes theN-terminal one-third of perR, including a region that encodesmost of the putative DNA-binding region of the protein (Fig. 5).The resulting mutant H $Delta$ Per proliferated as well as the wild typein aerobic growth conditions; however, no significant derepressionof the ahpC, gpoA, and mrgA reporter constructs were observedin H $Delta$ Per compared to the wild type (data not shown). These findingsindicate that, in contrast to what has been shown in B. subtilis,PerR does not appear to repress transcription of ahpC, gpoA, andmrgA in S. pyogenes. However, the PerR mutant was derepressedfor the inducible peroxide resistance response and survived lethalhydrogen peroxide challenge approximately 100 times better thanthe wild-type cells, even without preinduction with a sublethaldose of hydrogen peroxide or ethanol (Fig. 6). Interestingly,while the high level of resistance in the PerR mutant was notaffected by pretreatment with peroxide, an additional level ofresistance to lethal peroxide challenge could be induced by ethanol(Fig. 6). This observation is consistent with the observationthat ethanol consistently induced higher levels of resistanceto peroxide than did peroxide itself (see above) and suggeststhat the response induced by ethanol includes an additional regulatorycomponent independent of PerR.

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FIG. 5. Gene encoding PerR in S. pyogenes. The position and direction of perR are depicted relative to its neighbors in the genome as published by the Sanger Centre. This chromosomal structure is similar to that of the strains used in this study but is different from that of the M1 strain published by the University of Oklahoma. The percent amino acid identity and similarity to the closest match found by a TBlastN search are shown. Below is a partial alignment of the S. pyogenes perR gene with the B. subtilis homologue. Regions around the conserved putative helix-turn-helix DNA binding site and the putative metal-binding domain are shown. Two conserved CXXC putative metal-binding site motifs are shown in boxes. The 66-amino-acid region removed by deletion is indicated by the arrows. In the process of making the deletion, a valine and a tyrosine were replaced by a valine and an aspartic acid (underlined).

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FIG. 6. PerR is important for the inducible peroxide resistance response. The H $Delta$ Per mutant was compared to wild-type cells for the inducible peroxide resistance response. The relative survival was calculated as described in Fig. 4. Data for the wild type are shown in white; data for the H $Delta$ Per mutant are shown in black. The data represent the average of eight independent experiments. Error bars represent the standard error of the mean.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We employed functional genomics to investigate the mechanisms of defense against toxic oxygen species in the lactic acid bacteriumS. pyogenes. Using this approach, we have shown that while alkylhydroperoxide reductase (AhpC) and glutathione peroxidase (GpoA)contribute to resistance against methyl viologen and cumene hydroperoxide,neither enzyme is required for growth under aerobic conditionsor for the ability of S. pyogenes to mount an induced responseto peroxide stress. We have also found that the induced responseshares many characteristics with the $sigma$ ^B general stress response pathway but that S. pyogenes may lack $sigma$ ^B. On the other hand, we have discovered that PerR is a negativeregulator of the inducible peroxide resistance response. However,studies of ahpC and gpoA expression indicate that these genesare not induced under the conditions that lead to peroxide resistance,nor are they repressed by PerR. Collectively, these observationssuggest that in S. pyogenes PerR may repress genes encoding novelmechanisms of peroxideresistance.

Further support for the involvement of a novel mechanism comes from comparison of these data to similar studies conductedin the gram-positive bacterium B. subtilis. For example, B. subtilismutants deficient in either the catalase encoded by katA or theoxidoreductase encoded by ahpC grow normally under aerobic conditions(5). However, a katA ahpC double mutant exhibits a number ofstriking phenotypes, including slow growth in liquid media andaccelerated lysis on certain solid media (5). Significantly,while the Bacillus double mutant can grow as well as the wildtype under microaerobic conditions on rich medium, it grows verypoorly under these conditions on minimal medium and fails to growat all under normal aerobic conditions (5). Since S. pyogenesis naturally catalase deficient, the observation that the ahpCmutant is not defective for growth suggests that S. pyogenes hasalternative strategies for management of peroxidestress.

This possibility is also supported by the recent observation that S. mutans mutants lacking AhpC activity grow well aerobically(30). Furthermore, the fact that neither the gpoA mutant northe ahpC gpoA double mutant were defective for aerobic growthsuggests that glutathione peroxidase is not essential for thisphenotype. A recent report also showed that S. mutans mutantslacking AhpC or AhpF were not hypersensitive to cumene hydroperoxide(30). These data contrast with data showing that B. subtilisahpC mutants are 20 to 50 times more sensitive than the wild typeto cumene hydroperoxide (3). As mentioned above, our data indicatethat S. pyogenes ahpC gpoA mutants are only slightly more sensitiveto cumene hydroperoxide than is the wild type, again suggestinga possible alternate mechanism for peroxide resistance instreptococci.

While resistance to peroxide has not been well studied in most lactic acid species, mechanisms of aerotolerance appear tobe diverse among this family, and novel mechanisms of defenseagainst peroxide are not unprecedented. For example, one speciesof lactobacilli (Lactobacillus sake) produces a catalase thatutilizes heme scavenged from the organism's environment (35).A second lactobacillus species, Lactobacillus plantarum, harborsa pseudocatalase that uses two manganese atoms in place of hemeat its active site (32). In Enterococcus faecalis, a cystinylredox center-containing NADH peroxidase has been well characterized(55), and several oral streptococcal species, including Streptococcusgordonii, contain a gene with homology to the periplasmic thiolperoxidase of E. coli (7). As noted above, examination of theavailable genome information failed to reveal any clear homologuesof these other classes of peroxidases in S. pyogenes. However,given this diversity in mechanisms of achieving aerotoleranceamong lactic acid bacteria, it is not unreasonable to expect thatS. pyogenes may have evolved other unique and as-yet-uncharacterizedpathways for dealing with oxidativestress.

Identification of such alternative strategies will be facilitated by our studies of the PerR homologue in S. pyogenes. Eventhough the peroxidases known to be repressed by PerR in B. subtilis,namely, katA and ahpC, are not involved in the inducible responseto hydrogen peroxide in S. pyogenes, mutants lacking the PerRhomologue are constitutively resistant to hydrogen peroxide challenge.This finding suggests that PerR represses alternate genes importantfor the inducible response. MrgA has been shown to be essentialfor $sigma$ ^B-dependent resistance to oxidative stress in that species (2).However, our in vivo expression studies suggest that PerR is notan important regulator for MrgA in S. pyogenes. PerR itself isa transcription repressor with homology to the iron-sensitiveFur protein of E. coli (4) and binds to a well-conserved operatorsequence in its target promoters ("Per box") in B. subtilis (4,11). This sequence can be found in the promoter regions of genesrepressed by PerR in that species, including katA, ahpC, and mrgA.However, a search for Per boxes in ahpC and mrgA of S. pyogenesdid not reveal any such sequences, which is likely a significantobservation given that the putative DNA binding regions of PerRin S. pyogenes and B. subtilis are identical at 12 of 13 positions(4). Thus, the targets of PerR-dependent gene repression havenot yet been determined. Identification of such targets in S.pyogenes will provide further insight about potentially noveleffectors of protection against hydrogenperoxide.

The ability of ethanol to induce resistance to peroxide provides some insight into the regulation of this response. Stressresponses in prokaryotes are known to involve redundant and overlappingfunctions. For example, in E. coli, hydrogen peroxide exposureleads to the expression of a number of proteins, some of whichare also induced as part of the heat shock response. However,the peroxide response regulon also includes several proteins notregulated by the heat shock regulon (12, 19). In gram-positivebacteria, induction by ethanol is commonly used as a probe forregulation by the $sigma$ ^B-dependent general stress response (25, 53). This regulonis widely distributed among pathogenic gram-positive bacteria,including Staphylococcus and Listeria spp. (8, 54). However,our examinations using several different criteria, including examinationof the database for the $sigma$ ^B gene, $sigma$ ^B promoters, and genes which regulate $sigma$ ^B and PCR analyses, suggest that S. pyogenes may lack a clear homologueof $sigma$ ^B. In B. subtilis, a few stress response genes that are inducedby multiple stresses are regulated independently of $sigma$ ^B (29). These include the heat shock genes regulated by the CIRCEelement (29) and the genes for the various Clp-family proteasesthat are regulated by the recently described transcription repressorCtsR (15). However, there is no evidence that the genes regulatedby these responses specifically play major roles in resistancetoperoxide.

The ahpC and gpoA mutants are sensitive to high-level oxidative stress in the form of challenge with methyl viologen but arenot more sensitive to hydrogen peroxide in a disk diffusion orMIC assay. This apparent contradiction may be due to the factthat methyl viologen catalyzes the continuous production of superoxideand hydrogen peroxide in the culture medium, whereas exogenouslyadded hydrogen peroxide is reduced over time. In addition, ourfindings suggest that different mechanisms of resistance may beinvolved in protection from different levels of stress. The notionof a response tailored to the degree of stress is consistent withstudies suggesting that different levels of peroxide generatedifferent types of cellular damage in E. coli (28, 33). Peroxidekilling is bimodal with respect to peroxide concentration in E.coli, where it appears that low-level hydrogen peroxide exposureleads to DNA damage, whereas high levels of hydrogen peroxidemay directly oxidize some other cellular target (28, 33).Damage to different constituents would likely require differenttypes of repair and/or resistance mechanisms. The existence ofmultiple pathways in S. pyogenes is suggested by the observationthat ethanol can induce an additional degree of resistance inPerRmutants.

The regulation and manifestation of resistance to oxidative stress in S. pyogenes appear to involve several novel features.Since streptococcal lesions in tissue are highly inflammatoryand since the production of toxic oxygen species is an importantcomponent of the inflammatory response, the inducible responsemay serve as a virulence determinant that specifically allowsthe bacterium to survive oxidative stresses encountered in thehost environment. Further work is being undertaken to characterizethe components of this system and to understand its importancein bacterial survival andvirulence.

	ACKNOWLEDGMENTS

We thank Emil Unanue and Brian Edelson for the Listeria strains and Tim Foster for the Staphylococcus strains. We also thankBernard Beall for his interest in thesestudies.

This work was supported by Public Health Service grant AI38273 (M.G.C.) and NIH grant 5-T32-GM7200 (K.Y.K.).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Microbiology, Washington University School of Medicine, Box8230, St. Louis, MO 63110-1093. Phone: (314) 362-1485. Fax: (314)362-1232. E-mail: caparon{at}borcim.wustl.edu.

Present address: Yale University School of Medicine, New Haven, CT06520.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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1.	Altschul, S. F., W. Gish, W. Miller, E. W. Myers, and D. J. Lipman. 1990. Basic local alignment search tool. J. Mol. Biol. 215:403-410[CrossRef][Medline].
2.	Antelmann, H., S. Engelmann, R. Schmid, A. Sorokin, A. Lapidus, and M. Hecker. 1997. Expression of a stress- and starvation-induced dps/pexB-homologous gene is controlled by the alternative sigma factor sigmaB in Bacillus subtilis. J. Bacteriol. 179:7251-7256[Abstract/Free Full Text].
3.	Antelmann, H., S. Engelmann, R. Schmid, and M. Hecker. 1996. General and oxidative stress responses in Bacillus subtilis: cloning, expression, and mutation of the alkyl hydroperoxide reductase operon. J. Bacteriol. 178:6571-6578[Abstract/Free Full Text].
4.	Bsat, N., A. Herbig, L. Casillas-Martinez, P. Setlow, and J. D. Helmann. 1998. Bacillus subtilis contains multiple Fur homologues: identification of the iron uptake (Fur) and peroxide regulon (PerR) repressors. Mol. Microbiol. 29:189-198[CrossRef][Medline].
5.	Bsat, N., L. Chen, and J. D. Helmann. 1996. Mutation of the Bacillus subtilis alkyl hydroperoxide reductase (ahpCF) operon reveals compensatory interactions among hydrogen peroxide stress genes. J. Bacteriol. 178:6579-6586[Abstract/Free Full Text].
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