Deletion of the Alternative Sigma Factor sigma B in Staphylococcus aureus Reveals Its Function as a Global Regulator of Virulence Genes

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Journal of Bacteriology, September 1998, p. 4814-4820, Vol. 180, No. 18
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Deletion of the Alternative Sigma Factor $sigma$ ^B in Staphylococcus aureus Reveals Its Function as a Global Regulator of Virulence Genes

Ines Kullik,^* Philipp Giachino, and Thomas Fuchs

Institute for Medical Microbiology, University of Zürich, 8028 Zürich, Switzerland

Received 24 April 1998/Accepted 20 July 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results & Discussion References

A deletion of the sigB operon was constructed in three genetically distinct Staphylococcus aureus strains, and the phenotypesof the resulting mutants were analyzed. Compared to the correspondingwild-type strains, the $Delta$ sigB mutants showed reduced pigmentation,accelerated sedimentation, and increased sensitivity to hydrogenperoxide during the stationary growth phase. A cytoplasmic proteinmissing in the $Delta$ sigB mutants was identified as alkaline shockprotein 23, and an extracellular protein excreted at higher levelsin one of the $Delta$ sigB mutants was identified as staphylococcal thermonuclease.Interestingly, most sigB deletion phenotypes were only seen inS. aureus COL and Newman and not in 8325, which was found to containan 11-bp deletion in the regulator gene rsbU. Taken together,our results show that $sigma$ ^B is a global regulator which modulates the expression of severalvirulence factors in S. aureus and that laboratory strain 8325is a $sigma$ ^B-defective mutant.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results & Discussion References

The initial event during infection by the human pathogen Staphylococcus aureus is the expression of certain virulence genes.Virulence factors are required for colonization of host tissueand for protection against the host defense. Timely correct expressionof the virulence factors is essential for the establishment andmaintenance of an infection and represents a highly regulatedprocess (29). As a prerequisite, the microorganism has to recognizeand respond to certain signals provided by the host. Such signalscould be temperature (increases upon infection), peroxide (releasedby macrophages), pH shifts, or the presence or absence of specificcarbon or energy sources (24).

In bacteria, alternative sigma factors of RNA polymerase are known to play a crucial role in regulating gene expression uponmajor changes in the environment. We recently identified the alternativesigma factor $sigma$ ^B in S. aureus 8325 and showed that $sigma$ ^B is induced during stationary phase and upon heat shock (20).The corresponding sigma factor in B. subtilis is known to be itselftarget of a complex regulatory network, which controls gene expressionin response to certain stress and stationary-phase-specific signals(14). It has recently been shown that S. aureus $sigma$ ^B also has sigma factor activity in vitro and that transcriptionof the global regulator Sar in S. aureus is at least partiallycontrolled by $sigma$ ^B (8). Since the Sar protein represents a global regulator involvedin the expression of virulence genes (2, 4), it is temptingto speculate that $sigma$ ^B is directly or indirectly involved in the regulation of virulencegenes. To test this hypothesis, we constructed a sigB deletionin several staphylococcal backgrounds and analyzed the phenotypeof these mutants. Here we report that deletion of sigB causeda drastic phenotype in two of the three backgrounds tested andrevealed a natural $sigma$ ^B defect in strain 8325. Compared to strain COL, strain 8325 hasan 11-bp deletion in the gene encoding the $sigma$ ^B regulator RsbU (20, 36), which we suggest is the reason forthe $sigma$ ^B defect.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results & Discussion References

Bacterial strains, plasmids, culture conditions, and general methods. The bacterial strains and plasmids used in this study are listed in Table 1. S. aureus cells were routinely grown in Luria-Bertani(LB) medium at 37°C. Antibiotics were used at the following concentrations:for Escherichia coli, ampicillin at 100 µg ml¹; for S. aureus, erythromycin at 10 µg ml¹ and tetracycline at 10 µg ml¹. All DNA manipulations and handling of E. coli were performedin accordance with standard protocols (31). Manipulations withS. aureus were done as described earlier (20).

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TABLE 1. Strains and plasmids used in this study

Construction of plasmid pIK58, used to create a sigB deletion mutant. In a first step, we constructed the suicide vector pIKET by introducing appropriate antibiotic resistance cassettes into pBLSK(+),namely, the blunted 1.75-kb AvaI fragment with the ermB gene fromtransposon Tn551 in the EcoRV site of pBLSK(+), as well as theblunted 2.3-kb HindIII fragment with the tetK gene from pT181in the SmaI site. This plasmid cannot replicate in S. aureus,and erythromycin resistance can only be rescued by integrationof this plasmid into the chromosome. To provide sites for homologousrecombination, we cloned the S. aureus 1.1-kb NsiI fragment (downstreamregion of sigB) in the PstI site of the vector and the 1.7-kbrsbU'-containing HindIII fragment in the HindIII site, leadingto plasmid pIK58 (Fig. 1). Fifteen micrograms of this plasmidwas used to transform S. aureus RN4220 by electroporation witherythromycin for selection.

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FIG. 1. Physical map of the sigB operon of S. aureus and the construction of a sigB deletion using suicide plasmid pIK58. Open reading frames are depicted as rectangles with arrows indicating their orientation. The genes for ampicillin resistance (amp), erythromycin resistance (ermB), and tetracycline resistance (tetK) are indicated. Recognition sites for restriction enzymes are designated as follows: H, HindIII; N, NsiI; P, PstI; RV, EcoRV; Sm, SmaI. Sites in parentheses were destroyed during cloning. The bold line corresponds to S. aureus chromosomal DNA, the thin line corresponds to pBLSK(+) DNA, and the dashed line shows the cloning procedures. The crosses indicate sites of homologous recombination.

Lipase assay. To assay lipase activity, strains were grown for 12 h at 37°C in LB medium. Different dilutions of the culture supernatantswere tested for lipase activity by monitoring hydrolysis of p-nitrophenyl-caprylateat 405 nm as described elsewhere (27). Calculation of lipaseactivity was adjusted for cell density and expressed as a percentageof that of the respective wild-type parent. Since the levels oflipase production differed substantially among the three backgroundstested, dilutions of the supernatants were used to achieve a linearreaction in each case. Supernatants of strain 8325 were diluted20-fold, those of strain Newman were diluted 4-fold, and thoseof strain COL were used without dilution; the wild type and mutantswere always diluted equally. Lipase activity was also monitoredon LB agar plates containing 1% Tween 20 and 1% xylose.

Peroxide susceptibility testing. For disk assays, bacteria were plated on LB agar and a disk soaked with 10 µl of a 3% H₂O₂ solution was placed on the surface.Plates were incubated at 37°C for 48 h, and inhibition zones werecompared. MICs and MBCs of H₂O₂ were determined by broth microdilutionby using the National Committee for Clinical Laboratory Standardsprotocol (26) with serial dilutions of H₂O₂ (2.2 M to 0.125mM). Microtiter plates were incubated for 48 h at 37°C.

SDS-gel electrophoresis of protein, protein blotting, and N-terminal protein sequencing. Cellular or excreted proteins were separated by sodium dodecyl sulfate (SDS)-polyacrylamide gel electrophoresis by using standardprotocols (31). For analysis of excreted proteins, culture supernatantswere concentrated about 10- to 15-fold by using Microcon 10 spincolumns (Amicon Inc., Beverly, Mass.). Blotting of the proteinsonto polyvinylidene difluoride membranes was done as previouslydescribed (1), and N-terminal sequencing of the respectiveproteins was done by P. Hunziker in the Laboratory of Biochemistry,University of Zürich.

Construction of pIK64 for complementation of $Delta$ sigB strains. For complementation assays, we used vector pTX15, which contains the xylose-inducible promoter P_Xyl and a tetracycline resistancedeterminant (28). We first amplified the entire sigB gene byPCR and subcloned it into pBLSK(+). The correct sequence of thisfragment was confirmed by plasmid sequencing. We then subclonedthe sigB-containing BamHI/EcoRI fragment into the BamHI/EcoRIsites of pTX15 downstream of P_Xyl, leading to plasmid pIK64. SincepTX15 only contains a staphylococcal origin of replication, wedirectly transformed pIK64 into S. carnosus TM300 by using protoplasttransformation as previously described (13). pIK64 isolatedfrom S. carnosus was then used to transform S. aureus RN4220.From there, the plasmid was moved into wild-type and $Delta$ sigB mutantS. aureus by phage transduction as previously described (20).In those strains, P_Xyl and, therefore, expression of sigB wereinduced by adding 1% xylose to the medium. pIK64 could not beused for complementation of strain COL, since this strain naturallycontains a tetracycline resistance-encoding plasmid.

	RESULTS AND DISCUSSION

Top Abstract Introduction Materials & Methods Results & Discussion References

Construction of different sigB deletion mutants. To create a sigB deletion mutant by homologous recombination, we constructed pBLSK(+)-based suicide plasmid pIK58. This plasmidcontained two S. aureus DNA fragments flanking the region to bedeleted, as well as appropriate antibiotic resistance markersfor selection (Fig. 1). We transformed pIK58 into S. aureus RN4220and obtained approximately 100 erythromycin-resistant colonies.Since no plasmid could be isolated from those transformants, pIK58must have integrated into the chromosome through at least a singlecrossover in one of the two homologous regions. The colonies werereplica plated onto tetracycline, and three colonies were tetracyclinesensitive. This suggested that in these clones a double crossoverand, therefore, deletion of the sigB region had occurred (Fig.1). By using phage transduction and selection for erythromycinresistance, the deletion was transferred to three geneticallydifferent backgrounds: S. aureus 8325, COL, and Newman. S. aureus8325 represents a standard laboratory strain, whereas strain COLis a highly methicillin-resistant clinical isolate. Strain Newmanis characterized by a high level of clumping factor and is thereforeoften used in clumping or adhesion assays (9). After transduction,we isolated erythromycin-resistant and tetracycline-sensitiveclones in all three backgrounds. Southern blot hybridization usinga sigB-specific probe confirmed that sigB was deleted in all threestrains (data not shown). We characterized the phenotype of thosemutants as follows.

Reduced pigmentation. The first obvious phenotype of the sigB deletion mutants was their color on agar plates. Whereas colonies of the wild-typeparents of strains COL and Newman produced an orange pigment after24 h of incubation, the colonies of the respective sigB mutantswere unpigmented. In contrast, both wild-type strain 8325 andthe $Delta$ sigB mutant were unpigmented. Two major pigments are producedin S. aureus during stationary phase; the yellow carotenoid 4,4'-diaponeurosporeneis converted to the orange pigment staphyloxanthin after prolongedcultivation (34). The genes responsible for the biosynthesisof these pigments have been characterized (34, 35). By homology,we were able to identify a $sigma$ ^B-dependent promoter consensus sequence upstream of the staphyloxanthinbiosynthesis operon and thus propose that the conversion of 4,4'-diaponeurosporeneto staphyloxanthin during late stationary phase is $sigma$ ^B dependent in S. aureus. Interestingly, carotenoid synthesis inStreptomyces setonii is dependent on the $sigma$ ^B homologue CrtS (17).

Increased sedimentation and aggregation. The growth rates of all of the strains tested were unaffected by the sigB deletion, but strain Newman $Delta$ sigB exhibited acceleratedsedimentation when a culture grown overnight was left withoutagitation. In contrast to the wild-type parent, almost all cellsin the mutant culture were completely sedimented after less than1 h (Fig. 2A). Light microscopic analysis revealed that Newman $Delta$ sigB cells were clustered while wild-type cells were mostly separated(Fig. 2B). Electron microscopy confirmed close cell contact instrain Newman $Delta$ sigB (Fig. 2C). Close cell contact can be due toeither incomplete separation after cell division or secondaryinteraction of cell surface proteins, and the correct expressionand cellular localization of cell surface proteins is essentialfor successful colonization of surfaces by S. aureus (11, 12).However, the increased cell aggregation of the $Delta$ sigB mutant wasobserved only in strain Newman and not in strain COL or 8325.Strain Newman is known to produce high levels of clumping factor,a cell surface-associated fibrinogen receptor (23). It is possiblethat $sigma$ ^B modulates expression of the clumping factor or of other adhesins,which might lead to the observed cell aggregation also in cultures.

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FIG. 2. Comparison of liquid cultures of wild-type (wt) and $Delta$ sigB mutant (mut) forms of S. aureus Newman. (A) Sedimentation of a culture grown overnight is shown after 1 h without shaking. Overnight cultures were also analyzed by light microscope (×1,000 magnification) (B) or by electron microscope (C). In both cases, aggregation of the cells was visible. The arrows indicate areas of close contact between cells.

Decreased susceptibility to H₂O₂ during stationary phase. Since H₂O₂ represents an important stress factor for S. aureus during infection, we tested the H₂O₂ susceptibility of the $Delta$ sigB mutants in a disk diffusion assay. The diameters of theinhibition zones were the same in the wild type and $Delta$ sigB mutants,yet interestingly, after 48 h of incubation, we repeatedly observedwild-type colonies of strains COL and Newman close to the disk(Fig. 3). Those colonies were never observed with the sigB deletionmutants or with wild-type strain 8325. It was possible that thosecolonies represented highly H₂O₂-resistant second-site mutants.However, when they were reassayed for H₂O₂ susceptibility, theywere not highly resistant to H₂O₂, but the same growth patternas in the original assay was observed. This implies that the appearanceof such highly H₂O₂-resistant colonies in late stationary phase(48 h) is due to a transient effect, possibly an adaptive responseto H₂O₂. We also examined the MICs and MBCs of H₂O₂ (Table 2).For the wild-type COL and Newman strains, the MBC was higher thanthe MIC, whereas for COL $Delta$ sigB, Newman $Delta$ sigB, and wild-type and $Delta$ sigB 8325, the MICs and MBCs were identical. Thus, higher concentrationsof H₂O₂ are required to kill wild-type COL and Newman cells thanto inhibit growth, whereas in the respective sigB deletion mutants,as well as in strain 8325, the same concentration of H₂O₂ whichinhibits growth also kills the cells. This is in accordance withthe results seen in the zone assay, where after 48 h only wild-typeCOL and Newman cells could again grow after being initially inhibited.Taken together, these data suggest that in S. aureus growth athigh concentrations of peroxide during late stationary phase requires $sigma$ ^B.

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FIG. 3. Comparison of the H₂O₂ susceptibilities of wild-type (wt) and $Delta$ sigB mutant (mut) strains of S. aureus in a disk diffusion assay after 48 h. The primary inhibition zones of all strains were comparable, but wild-type strain COL and Newman colonies growing close to the central H₂O₂ disk were visible after 48 h of incubation.

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TABLE 2. Susceptibilities of S. aureus sigB mutant strains and their wild-type parents to H₂O₂

H₂O₂ is detoxified by the enzyme catalase, which is considered to be an important virulence factor in S. aureus. Catalaseprotects the cells from the oxidative burst released from hostmacrophages upon infection, and in S. aureus, a correlation betweencatalase activity and virulence has been observed (16, 22).In E. coli, expression of the two catalase genes is regulatedby the stationary-phase sigma factor $sigma$ ^S (15, 25), and in B. subtilis, one catalase gene has beenshown to be regulated by $sigma$ ^B (10). S. aureus also appears to have multiple catalase activities(7), and since the growth of S. aureus at high concentrationsof H₂O₂ in late stationary phase was $sigma$ ^B dependent, we suggest that expression of at least one of thecatalases is regulated by $sigma$ ^B. Preliminary data from catalase activity stains of native proteingels with total protein from S. aureus wild-type and $Delta$ sigB strainsrevealed the existence of at least two bands with catalase activity,of which one was less abundant in the $Delta$ sigB strains (data notshown). However, further biochemical analysis is required to definethose activities.

Expression of Asp23 and thermonuclease is affected by the sigB deletion. By using SDS-polyacrylamide gel electrophoresis, we compared the total protein expression patterns and the levels of excretedprotein of the wild-type and $Delta$ sigB strains (Fig. 4). The patternsof total protein expression of the wild-type and mutant strainswere very similar. However, one very abundant protein of about23 kDa was clearly missing in the $Delta$ sigB mutants of strains COLand Newman and also in wild-type 8325 (arrow in Fig. 4A). N-terminalsequencing of this protein revealed the amino acid sequence MTVDNNKAKQAYDNQ,which shows 100% identity with the first 15 amino acids of alkalineshock protein 23 (Asp23) of S. aureus. The asp23 gene was previouslyfound to encode a 169-amino-acid protein with an unknown functionand a molecular mass of 19.2 kDa (21). Although the molecularmass of Asp23 is predicted to be 19.2 kDa, it reveals an apparentmolecular mass of 23 kDa on a protein gel. It was furthermoredemonstrated that expression of Asp23 is strongly induced upona pH upshift to 10 (21). The transcriptional start site of asp23has been mapped (21), and upon examination of the sequence,we found a perfect $sigma$ ^B-dependent promoter consensus sequence, instead of the proposed $sigma$ ^A promoter, at the correct distance from the transcriptional startof the gene. These observations strongly suggest that asp23 isa $sigma$ ^B target in S. aureus. In growth assays, the $Delta$ sigB mutant strainswere slightly more sensitive to a pH upshift from 7 to 10 duringexponential growth phase (data not shown). However, the functionof Asp23 in S. aureus and its possible role in permitting S. aureusto grow at high pHs remain to be determined.

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FIG. 4. SDS-polyacrylamide gel electrophoresis analysis of wild-type and $Delta$ sigB mutant S. aureus strains. In A, about 20 µg of total cellular protein per lane was analyzed; in B, about 5 µg of excreted protein per lane was analyzed. Samples were analyzed as follows: lanes 1 and 2, strain 8325; lanes 3 and 4, strain COL; lanes 5 and 6, strain Newman. Extracts in lanes 1, 3, and 5 were from the wild-type parent, and those in lanes 2, 4, and 6 were from the corresponding $Delta$ sigB mutant. In C, 10 µg of total cellular protein per lane from the following strains was analyzed: lanes 1 and 2, strain 8325 wild type; lanes 3 and 4, strain 8325 $Delta$ sigB; lanes 5 and 6, strain Newman wild type; lanes 7 and 8, strain Newman $Delta$ sigB. Lanes 1, 3, 5, and 7 were complemented with plasmid pIK64. A protein standard was loaded in lanes M. The arrows in A and C indicate the protein identified as Asp23. The arrow in B indicates the protein identified as staphylococcal thermonuclease.

On gels of the excreted proteins of S. aureus, the amount and pattern of excreted proteins varied significantly among wild-typestrains 8325, COL, and Newman (Fig. 4B). Comparison of each wild-typeparent with the respective $Delta$ sigB mutant revealed three classesof proteins: (i) those which were identical in the wild type andthe mutant, (ii) those which were less abundant in the mutant,and (iii) those which were enhanced in the mutant. We determinedthe N-terminal sequence of a 23-kDa protein from $Delta$ sigB mutantstrains COL and Newman (arrow in Fig. 4B) and in both cases obtainedthe amino acid sequence SQTDNGVNR, which showed 100% identitywith amino acids 64 to 72 of the staphylococcal thermonuclease(5, 6, 18). Staphylococcal thermonuclease is an excretedtoxin of 231 amino acids with a molecular mass of 25.5 kDa. Aminoacids 1 to 63 serve as a signal peptide which is cleaved off afterprotein export. Therefore, the mature excreted protein beginswith amino acid 64, which is exactly where the homology to ourprotein sequence starts. Thermonuclease was hardly detectablein wild-type and mutant 8325 but highly abundant in both wild-typeand $Delta$ sigB mutant strain Newman. Interestingly, in strain COL,thermonuclease was more prominent in the $Delta$ sigB mutant than inthe wild type, indicating that in this strain $sigma$ ^B has a negative effect either on protein expression or on exportof this protein into the medium. Taken together, our data indicatethat deletion of $sigma$ ^B can have both positive and negative effects on certain proteins.It also shows that additional strain-specific factors may existwhich modulate $sigma$ ^B-dependent regulation in the respective background.

Increased lipase activity. Lipase represents an important virulence factor that is excreted mainly during stationary growth phase and can easily be assayedeither on plates or in liquid culture supernatants. On plates,we observed that all of the sigB deletion strains studied producedmore lipase than did their respective wild-type parents (datanot shown). This effect was confirmed by a quantitative assayof culture supernatants. Interestingly, the levels of lipase expressionvaried significantly among the three wild-type strains, with strain8325 showing the highest activity and strain COL showing the lowestactivity. Since we focused on the effect of the sigB deletionin each case, the lipase activity of each wild-type strain wasset as 100% and the $Delta$ sigB mutant levels were compared with thoseof the corresponding parents (Table 3). For strains 8325 andCOL, lipase production was about 1.5 times as high in the $Delta$ sigBmutant as in the parent, and for strain Newman, mutant lipaseactivity was increased three- to fourfold. Those values were highlyreproducible and were confirmed in four independent assays. Hence,we speculate that lipase production or excretion during stationarygrowth phase is negatively regulated by $sigma$ ^B or by a $sigma$ ^B-dependent factor.

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TABLE 3. Lipase activities of S. aureus sigB mutant strains and their wild-type parents

Complementation of $Delta$ sigB mutants restores pigmentation and Asp23 production. To prove that the observed phenotypes of the mutants are due to the deletion of sigB itself, we complemented the mutants withplasmid pIK64, carrying the sigB gene under control of the xylose-induciblepromoter P_Xyl. pIK64 was introduced into the wild-type and $Delta$ sigBmutant forms of strains 8325 and Newman but could not be usedin strain COL because of the overlapping tetracycline resistanceencoded by plasmid pIK64 and a plasmid naturally present in thisbackground. When $Delta$ sigB strains 8325 and Newman containing pIK64were grown in medium with xylose, the formerly pigmentless strainsproduced a very intense orange pigment, even during exponentialgrowth phase and not only in late stationary phase. In contrast,without xylose in the medium, no such pigment was produced. Theseresults show that (i) sigB alone restores pigmentation in thepigmentless $Delta$ sigB mutants and (ii) overexpression of plasmid-encodedsigB causes overexpression of the orange pigment staphyloxanthineven much earlier than in the wild-type situation. Therefore,we conclude that the operon for staphyloxanthin biosynthesis isa direct target of $sigma$ ^B. pIK64 even caused orange pigmentation in otherwise pigmentlesswild-type 8325, meaning that the missing pigmentation in thisstrain is not due to a loss or defect of the pigmentation genesbut rather to a nonfunctional $sigma$ ^B protein, most likely due to a defective RsbU protein, as describedlater in the report.

We also analyzed the expression of the protein Asp23 in the complemented mutants (Fig. 4C). Addition of pIK64 and xylose restoredAsp23 expression in wild-type 8325, $Delta$ sigB 8325, and $Delta$ sigB Newman(lanes 1, 3, and 7). In wild-type strain Newman, the presenceof pIK64 even slightly increased the amount of Asp23 (lane 5).These results support our assumption that asp23 is also a directtarget of $sigma$ ^B. Taken together, the complementation data prove that deletionof $sigma$ ^B alone leads to the observed phenotypes in the mutants described.

Deletion of 11 bp of rsbU in strain 8325 and derivatives. We previously found that strain 8325 contains an 11-bp deletion in the rsbU gene in comparison to the B. subtilis sequenceand also in comparison to the sigB sequence in S. aureus COL (20).To test whether this deletion was present in other 8325 derivativesas well, we performed PCR with oligonucleotides flanking the deletionsite. PCR should give rise to a 77-bp fragment in the wild typeand a 66-bp fragment in a mutant with an 11-bp deletion. Two independent8325 strains (lanes 1 and 5) and strain RN4220 (an 8325 derivative)(lane 3) had an 11-bp deletion, whereas strains COL and Newman(lanes 2 and 4) had no deletion (Fig. 5).

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FIG. 5. PCR of different S. aureus strains using primers flanking the 11-bp deletion in the rsbU gene. Amplification products were analyzed on a 4% agarose gel as follows: lane 1, strain 8325; lane 2, strain COL; lane 3, strain RN4220, lane 4, strain Newman; lane 5 independent source of strain 8325. A 100-bp DNA ladder was loaded in lane M as a molecular size marker.

In B. subtilis, an intact RsbU phosphatase is required for full $sigma$ ^B activity under stress conditions (32, 33). Therefore, itis to be expected that S. aureus $sigma$ ^B can only be activated under the respective stress conditionsin strains with functional RsbU. Consequently, it is plausiblethat deletion of $sigma$ ^B results in a mutant phenotype only in strains with intact RsbU.

Wild-type strain 8325 resembles the COL and Newman $Delta$ sigB mutants with respect to Asp23 expression, H₂O₂ susceptibility, andpigmentation. Therefore, we suggest that strain 8325 representsa natural $sigma$ ^B-defective mutant most probably due to the 11-bp deletion in thersbU gene. In contrast, $Delta$ sigB strain 8325 does show a mutant phenotypewith respect to lipase production during stationary growth phase,where $sigma$ ^B might activate a negative effector. From work with B. subtilis,it is known that $sigma$ ^B can be activated via two pathways: during exponential phase byan RsbU-dependent pathway and by an RsbU-independent pathway duringstationary phase (33). We propose that to control lipase productionduring stationary phase, $sigma$ ^B does not require stress induction via RsbU but can still be activatedduring stationary phase in an RsbU-independent way.

In summary, we have demonstrated that a sigB deletion in S. aureus produces a pleiotropic phenotype. Our results suggest thatasp23 and the operon for staphyloxanthin biosynthesis are directtargets of $sigma$ ^B in S. aureus. In B. subtilis, $sigma$ ^B is a stationary-phase- and stress-specific sigma factor and severaltarget genes are known to be $sigma$ ^B dependent. However, in many cases, the function of the targetgenes is unknown, and a sigB mutation has no clear phenotype.Stress survival does also not appear to be impaired in the mutants(14). $sigma$ ^B may not be essential for survival but might give a competitiveadvantage under specific environmental conditions. In a pathogenlike S. aureus, expression of virulence genes is not essentialbut enables the cells to colonize and survive in human hosts,who serve as a specialized ecological niche. Several of the functionswhich we have demonstrated to be modulated by $sigma$ ^B in S. aureus, such as peroxide resistance, possibly alkali stressresponse, cell aggregation, or lipase and thermonuclease production,may play an important role during infection. In addition, expressionof the global regulator Sar is $sigma$ ^B dependent (8). The Sar protein is required for expressionof the regulator Agr (3), which, in turn, affects the expressionof a variety of virulence factors (30). Thus, we suggest thatS. aureus $sigma$ ^B is a stress- and stationary-phase-specific global regulator whichis directly and indirectly involved in the expression of virulencegenes. We predict that the identification of additional $sigma$ ^B-dependent target genes will provide insight into the regulatorypathways controlling the process of infection.

	ACKNOWLEDGMENTS

We thank Ursula Hardegger for excellent technical assistance and Brigitte Berger-Bächi for fruitful discussions. We alsothank Peter Hunziker, Institute of Biochemistry, University ofZürich, for protein sequencing. This work was done in the laboratoryof F. H. Kayser, whose generous support is gratefully acknowledged.

P.G. was supported by NF grant 31-46762.96 of the Schweizerischer Nationalfonds.

	FOOTNOTES

^* Corresponding author. Present address: Pharmacia & Upjohn AG, Lagerstr. 14, 8600 Dübendorf, Switzerland. Phone: 41-1-80281 65. Fax: 41-1-802 81 49. E-mail address: ines.kullik-stax{at}eu.pnu.com.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results & Discussion
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Deletion of the Alternative Sigma Factor B in Staphylococcus aureus Reveals Its Function as a Global Regulator of Virulence Genes

Deletion of the Alternative Sigma Factor $sigma$ ^B in Staphylococcus aureus Reveals Its Function as a Global Regulator of Virulence Genes