The VirR Response Regulator from Clostridium perfringens Binds Independently to Two Imperfect Direct Repeats Located Upstream of the pfoA Promoter

doi:10.1128/JB.182.1.57-66.2000

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Journal of Bacteriology, January 2000, p. 57-66, Vol. 182, No. 1
0021-9193/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The VirR Response Regulator from Clostridium perfringens Binds Independently to Two Imperfect Direct Repeats Located Upstream of the pfoA Promoter

Jackie K. Cheung and Julian I. Rood^*

Bacterial Pathogenesis Research Group, Department of Microbiology, Monash University, Clayton 3800, Australia

Received 21 July 1999/Accepted 7 October 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Regulation of toxin production in the gram-positive anaerobe Clostridium perfringens occurs at the level of transcriptionand involves a two-component signal transduction system. The sensorhistidine kinase is encoded by the virS gene, while its cognateresponse regulator is encoded by the virR gene. We have constructeda VirR expression plasmid in Escherichia coli and purified theresultant His-tagged VirR protein. Gel mobility shift assays demonstratedthat VirR binds to the region upstream of the pfoA gene, whichencodes perfringolysin O, but not to regions located upstreamof the VirR-regulated plc, colA, and pfoR genes, which encodealpha-toxin, collagenase, and a putative pfoA regulator, respectively.The VirR binding site was shown by DNase I footprinting to bea 52-bp core sequence situated immediately upstream of the pfoApromoter. When this region was deleted, VirR was no longer ableto bind to the pfoA promoter. The binding site was further localizedto two imperfect direct repeats (CCCAGTTNTNCAC) by site-directedmutagenesis. Binding and protection analysis of these mutantsindicated that VirR had the ability to bind independently to thetwo repeated sequences. Based on these observations it is postulatedthat the VirR positively regulates the synthesis of perfringolysinO by binding directly to a region located immediately upstreamof the pfoA promoter and activatingtranscription.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Bacteria use two-component signal transduction systems to respond to changes in environmental factors such as nutrient availability,temperature, osmolarity, pH, and oxygen tension (1). Theseregulatory networks usually consist of a membrane-associated sensorhistidine kinase and its cognate response regulator, which communicateby a phosphorelay cascade that generally leads to the modulationof gene expression (56). The majority of two-component signaltransduction systems have been identified in prokaryotes, butthey have also been found in some eukaryotes (21). The phosphorelayprocess usually involves the detection of a specific environmentalstimulus, which induces the autophosphorylation of the sensorkinase at a conserved histidine residue located in the cytoplasmicC-terminal region (38). This domain also contains conservedmotifs that are involved in ATP binding and kinase activity (40).Once phosphorylated, it can act as phosphodonor for its cognatecytoplasmic response regulator. The N-terminal domain of the responseregulator catalyzes the transfer of the phosphoryl group fromthe histidine residue to a conserved aspartate residue, whichin essence activates the response regulator so that it is ableto bind to its target DNA and subsequently modulate gene expression(38).

Clostridium perfringens is a gram positive anaerobic bacterium that is the causative agent of gas gangrene, or clostridialmyonecrosis, and is characterized by its ability to produce manyextracellular toxins and enzymes (44). Of these toxins, alpha-toxin(phospholipase C) and perfringolysin O (theta-toxin) have beenimplicated in gas gangrene (2, 13, 54). The productionof these toxins and collagenase (kappa-toxin), protease, and sialidasehas been shown to be regulated by a two-component signal transductionsystem that comprises the VirS sensor histidine kinase and theVirR response regulator, which are encoded by the virS and virRgenes, respectively (27, 48). Mutation or inactivation ofeither virR or virS alters the ability to produce the varioustoxins (3, 27, 48). It has been proposed that when thetransmembrane region of VirS detects an as yet unidentified environmentalor growth phase stimulus, it autophosphorylates at His-255 andthen acts as a phosphodonor for the phosphorylation of Asp-57of VirR. The phosphorylated VirR protein positively regulatesthe transcription of its target genes either directly or by activatingthe transcription of other regulatory genes (3, 27, 43).

Comparison of the putative amino acid sequence of VirR with those of other response regulators revealed significant sequencesimilarity in the N-terminal region (27), in particular twoconserved aspartate residues and conserved lysine and glutamateresidues, all of which are proposed to form the catalytic domainwhere phosphorylation occurs (4, 53, 55, 58). Studieswith other response regulators have shown that they often activatetranscription by binding to a promoter region upstream of thetarget gene. However, unlike those of many response regulators,the C-terminal domain of VirR does not contain any DNA bindingmotifs such as a helix-turn-helix motif (38, 39) or a helix-loop-helixdomain (29). Consensus binding sequences have been identifiedupstream of the genes regulated by other response regulators suchas OmpR (15, 16, 41), PhoP (23, 24), and AlgR (35,36). However, no common nucleotide sequences that could actas consensus binding sites were identified upstream of the VirR-regulatedgenes (3).

The objectives of this study were to determine if VirR could bind to the promoter regions of its target genes and if so toidentify its precise binding sites. The initial target regionsthat were tested were located upstream of the VirR-regulated plc,colA, pfoR, and pfoA genes, which, respectively, encode alpha-toxin,collagenase, the putative regulatory protein PfoR, and perfringolysinO. The results show that VirR binds to two imperfect direct repeatslocated upstream of the pfoAgene.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Strains, plasmids, and growth media. All bacterial strains and plasmids used in this study are listed in Table 1. Escherichia coli strains were cultured at 37°Cin 2× YT broth or agar medium or SOC broth (46) supplementedwith ampicillin (100 µg ml¹).

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TABLE 1. Relevant strains and plasmid used in this study

Molecular techniques. Plasmid DNA was routinely isolated by an alkaline lysis method (37). When used for sequencing, DNA was isolated by the modifiedmini-alkaline-lysis/polyethylene glycol precipitation procedureoutlined in the PRISM Ready Reaction Dye Deoxy terminator cyclesequencing kit protocol (Applied Biosystems, Foster City, Calif.).Rubidium chloride-competent E. coli cells were prepared and transformedas previously described (14). Transformation of electrocompetentE. coli cells (52) was carried out with a Bio-Rad (Hercules,Calif.) Gene Pulser in 0.1-ml cuvettes under conditions outlinedby themanufacturer.

PCR amplification was performed with Taq DNA polymerase (Boehringer GmbH, Mannheim, Germany) and a 0.5 µM concentration ofeach primer (Table 2) in a total volume of 100 µl. Reactionswere carried out in a GeneAmp PCR System 2400 (Perkin-Elmer Corp.,Foster City, Calif.), and the 94°C denaturation (1 min), 50°Cannealing (2 min), and 72°C extension (3 min) steps were carriedout for 30 cycles. The final cycle consisted of 2 min of annealingand 5 min of extension at the temperatures indicated above. Alloligonucleotide primers used (Table 2) were synthesized on anApplied Biosystems 394 DNA/RNA synthesizer.

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TABLE 2. Oligonucleotide primers

Nucleotide sequence analysis was carried out with a PRISM Big Dye terminator cycle sequencing Ready Reaction kit and AmpliTaqpolymerase FS (Applied Biosystems) in accordance with the manufacturer'sinstructions. Sequencing samples were resolved and analyzed ona 373 DNA STRETCH sequencer (Applied Biosystems). Sequence analysiswas performed with Sequencher 3.0 software (GeneCodes Corp., AnnArbor, Mich.).

Construction of recombinant plasmids. Plasmid DNA was digested with restriction endonucleases as specified by the manufacturers (Boehringer GmbH and New EnglandBiolabs, Beverly, Mass.). Insert and vector DNA was isolated withthe BRESA-CLEAN nucleic acid purification kit (Bresatec, Adelaide,Australia). When required, insert DNA and vector DNA were treatedwith T4 polynucleotide kinase (Promega Corp., Madison, Wis.) oralkaline phosphatase (Boehringer GmbH) as specified by the manufacturers.Vector and insert DNA was ligated with T4 DNA ligase (3 U µl¹; Promega Corp.) at 16°Covernight.

The plasmid pJIR1342 was constructed as follows to facilitate overexpression and purification of a His-tagged VirR protein.The 711-bp virR gene was amplified by PCR from pJIR870 (Table1) with oligonucleotides 2799 and 2798 (Table 2). These primersintroduced BamHI and EcoRI sites at the 5' and 3' ends of thePCR-generated virR gene, respectively, and enabled the amplifiedgene to be inserted into the BamHI and EcoRI sites of the expressionvector pRSET A (Invitrogen, Carlsbad, Calif.) (Table 1) in thecorrect reading frame. Sequence analysis confirmed the in-frameinsertion and confirmed that no mutations had been introducedbyPCR.

To facilitate DNase I footprinting and site-directed mutagenesis, plasmid pJIR1546 was constructed by cloning a 278-bp PCRproduct containing the pfoA promoter region into the SmaI siteof pUC18 (60). The PCR product was obtained by amplificationwith oligonucleotides 6565 and 6566 (Table 2). Similarly, pJIR1781was constructed by cloning a 342-bp PCR product, from which theVirR binding site had been deleted, into the SmaI site ofpUC18.

Expression and purification of His-tagged VirR. E. coli BL21(DE3)(pLysS) cells (Novagen, Madison, Wis.) harboring pJIR1342 were cultured overnight at 37°C in 2× YT brothsupplemented with ampicillin (100 µg ml¹) before being diluted 1 in 10 with the same medium. After incubationat 37°C for 1 h, the expression of His-tagged VirR was inducedwith 2 mM isopropyl- $beta$ -D-thiogalactopyranoside (IPTG) (Progen,Darra Q, Australia) at 37°C for 30 min to 1 h. Cells were harvestedby centrifugation at 16,300 × g for 10 min, resuspended in lysisbuffer (20 mM Tris-HCl, 0.3 M NaCl, 10% glycerol, 5 mM imidazole,pH 7.9) and lysed by passage twice through a French press. Cellulardebris was removed by centrifugation at 4°C as described above.The supernatant was applied to a Talon (Clontech, Palo Alto, Calif.)affinity column consisting of 1 ml of bed resin which had beenpreviously equilibrated with lysis buffer. Proteins were allowedto bind for 1 h at 4°C while rotating, followed by three washeswith 5 ml of lysis buffer. His-VirR was eluted with 5 ml of elutionbuffer (20 mM Tris-HCl, 0.3 M NaCl, 10% glycerol, pH 7.9) supplementedwith 20, 60, 100, or 200 mM imidazole, and 1-ml fractions werecollected. Samples of each fraction were mixed with gel loadingbuffer and subjected to sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) (22). The SDS-12% PAGE gels werestained with Coomassie brilliant blue essentially as describedpreviously (46). Fractions containing highly purified VirR protein(the 20 and 60 mM imidazole fractions) were then pooled and dialyzedovernight in dialysis buffer (100 mM NaCl, 20 mM Tris [pH 7.5],1 mM EDTA, 10% glycerol) at 4°C. The protein was concentratedby use of a Biomax-10 Ultrafree-15 centrifugal filter device (MilliporeCorp., Bedford, Mass.) and stored at $-$ 70°C. Protein concentrationswere determined by use of the BCA protein assay kit (Pierce, Rockford,Ill.).

Gel mobility shift assays. PCR-generated target DNA fragments were labelled with digoxigenin-11-ddUTP (DIG) at their 3' termini with the DIG gel shiftkit (Boehringer GmbH) as described by the manufacturer. Bindingreactions were carried out in a total volume of 20 µl, and reactionmixtures consisted of 4 µl of binding buffer (DIG gel shift kit),1 µg of poly(dI-dC), 0.1 µg of poly-L-lysine, 15 fmol of DIG-labelledtarget DNA, 1 or 2 µg of purified VirR, and sterile distilledwater. Binding reaction mixtures were incubated at room temperaturefor 15 min before the addition of gel loading buffer (suppliedwith the kit) that did not contain bromophenol blue. Reactionmixtures were then immediately loaded onto a preelectrophoresed4% native 0.25× TBE (22.3 mM Tris, 22.3 mM boric acid, 0.5 mMEDTA, pH 8.0) polyacrylamide gel, alongside a control lane containinggel loading buffer with bromophenol blue. Samples were separatedat 170 V and 4°C until the blue dye front was on the verge ofrunning off the gel. The gel was then capillary transferred ontoan Nylon⁺ membrane (Amersham Life Science, Buckinghamshire, United Kingdom)as described for Southern blots (46), with 0.25× TBE as thetransfer buffer. Following overnight transfer at room temperature,the membrane was soaked in 10× SSC (1.5 M NaCl, 0.15 M sodiumcitrate, pH 7.0) and then cross-linked for 3 min at 312 nm witha Hybaid cross-linker (Integrated Sciences, Melbourne, Australia).Chemiluminescent detection of the bound probe was carried outas described by the manufacturer. The chemiluminescent signalswere recorded by exposure to X-ray film (Fuji, Tokyo, Japan) atroomtemperature.

To quantitate the concentration dependence of VirR binding, the 183-bp pfoA target fragment was end-labelled with [ $alpha$ -³²P]dATP by terminal transferase (Boehringer GmbH) in accordancewith the manufacturer's instructions. Labelled DNA was used ingel mobility shift assays as described for DIG-labelled DNA, withthe exception that the target fragment was incubated with variousconcentrations of VirR. Following electrophoresis, the acrylamidegel was vacuum dried and then exposed overnight to a phosphorscreen (Molecular Dynamics, Sunnyvale, Calif.). Quantitative datawere obtained with the STORM 690 PhosphorImager (Molecular Dynamics)with ImageQuant software (MolecularDynamics).

DNase I footprinting. The DNA probes were generated by PCR with oligonucleotide primers that had been end-labelled with [ $gamma$ -³²P]ATP by T4 polynucleotide kinase as described previously (19).For protection studies on the sense and antisense strands, PCRprimers 6519 and 5126, respectively, were labelled. The amplifiedlabelled products were isolated with the BRESA-CLEAN nucleic acidpurification kit and quantitated in a Wallac 1410 scintillationcounter (Wallac Oy, Turku,Finland).

Binding reactions were carried out in a total volume of 80 µl. The reaction mixtures consisted of the labelled DNA probe (25,000cpm µl¹), 16 µl of binding buffer [100 mM HEPES (pH 7.6), 50 mM (NH₄)₂SO₄,5 mM 1,4-dithiothreitol, 1% (wt/vol) Tween 20, 150 mM KCl], 1µg of poly(dI-dC), and the appropriate amount of purified VirR.Following incubation for 15 min at room temperature, MgCl₂ wasadded to a final concentration of 4 mM prior to DNase I digestion.The target DNA in the no-VirR control was digested with 1 U ofRQ1 RNase-free DNase (Promega); 2 U of RQ1 DNase was added tothe reaction mixtures containing VirR. The samples were partiallydigested at room temperature for 1 min, and then the reactionwas stopped by the addition of phenol (saturated with 1 mM Tris-0.1mM EDTA, pH 8.0). The footprinting reaction products were thenextracted and precipitated as described before (19), with theexception that the reaction products were resuspended in 3 µlof Stop solution from the T7 sequencing kit (Pharmacia Biotech,Uppsala, Sweden) and run on an 8% sequencing gel. To localizethe DNase I footprint, sequencing reaction products generatedby the T7 sequencing kit with primers 6519 or 5126 were run alongsidethe footprinting reactionproducts.

Deletion by SOE PCR. Deletion of the VirR binding site in the pfoA promoter region was achieved by the splice overlap extension (SOE) PCR method(17), with a few modifications. Briefly, two separate PCR productswere generated with pTS302 (Table 1) as the template and theprimer pairs 6926 and 7352 and 6927 and 6928 (Table 2). Theseproducts, which contain complementary sequences, were isolatedwith the QIAquick gel extraction kit (Qiagen GmbH, Hilden, Germany).The purified products were then spliced together by PCR with primers6926 and 6928; the 91°C denaturation (1 min), 37°C annealing (1min), and 72°C extension (2 min) steps were carried out for 30cycles. The final cycle consisted of 1 min of denaturation andannealing and 5 min of extension at the temperatures indicatedabove. The 2,080-bp SOE PCR product was then used as the templatein a PCR with primers 6926 and 5126. The resultant 342-bp productwas completely sequenced to ensure that the appropriate regionhad been deleted and to confirm that no other mutations had beenintroduced.

Site-directed mutagenesis. Site-directed mutagenesis was carried out by the unique site elimination method (11) with a U.S.E. mutagenesis kit (PharmaciaBiotech) by a modification of the manufacturer's instructions.The second round of restriction enzyme selection was performedin a total volume of 20 µl, and the digested DNA was used to transformrubidium chloride-treated competent E. coli cells. These cellswere heat shocked at 37°C for 2 min before inoculation into SOCbroth. Plasmids were screened by restriction analysis, and thedesired mutations were confirmed by nucleotide sequence analysis.All mutated DNA inserts were completely sequenced to confirm thatno additional mutations had beenintroduced.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Overexpression and purification of His-tagged VirR. To overexpress the VirR protein, the virR gene was amplified by PCR and cloned into expression vector pRSET A. Sequence analysisof the resultant plasmid, pJIR1342, confirmed that no mutationshad been introduced into the virR gene. IPTG induction in E. coliBL21(DE3)(pLysS)(pJIR1342) cells and Western blotting with anantibody specific for the fused vector-specific leader regionshowed that these cells produced an immunoreactive protein ofthe same size as the expected N-terminal fusion protein (His-VirR)(data not shown). However, even after 4 h of IPTG induction, thelevels of expression were not sufficient to observe this proteinin crude extracts separated by SDS-PAGE and stained with Coomassieblue (Fig. 1). Nonetheless, the presence of a six-His tag at theN terminus of the fusion protein facilitated the purificationof the protein under native conditions by metal ion chelationchromatography with Talon affinity resin. Cells used in purificationwere induced for 30 min to 1 h, since a time course experimentdemonstrated that a longer induction period resulted in significantprotein degradation (data not shown). The purified protein wasvisualized on Coomassie-stained SDS-12% PAGE gel (Fig. 1) andwas shown to migrate in accordance with its estimated molecularsize of 33 kDa.

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FIG. 1. Purification of VirR. Low-molecular-weight standards (Pharmacia Biotech), in kilodaltons, are shown adjacent to the gel. Lanes 1 and 3, uninduced whole-cell extracts from cells harboring the vector pRSET A or pJIR1342, respectively; lanes 2 and 4, postinduction (4 h) whole-cell extracts from cells carrying the vector or pJIR1342, respectively; lane 5, His-VirR purified from cells induced for 30 to 60 min with IPTG (arrow).

Does VirR bind to the target gene regions? To identify possible VirR binding sites, purified VirR was used in gel mobility shift experiments with upstream promoter regionsof the plc, colA, pfoA, and pfoR genes. In previous studies, thetranscription of these genes was found to be affected by mutationsin either virR or virS (3, 27, 49). The upstream regionswere amplified by PCR (Table 2) and labelled with DIG. Each ofthe target fragments contained the VirR-dependent promoter ofthe respective gene (Fig. 2), with the exception of pfoR, sinceits promoter has not yet been identified.

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FIG. 2. Gel mobility shift analysis of target gene regions. Shown are the results of gel mobility shift assays using plc (A), colA (B), pfoR (C), and pfoA (D) gene regions. These regions are shown in the schematic above each gel shift result, with the rectangular boxes representing the respective genes. The direction of transcription is shown by arrows from each promoter (P). The DNA fragments used in the assays are shown by the solid bars, and their respective sizes (in base pairs) are shown above the bars. (A and B) Lane 1, no-VirR control; lanes 2 and 3, DIG-labelled target DNA incubated with 1 and 2 µg of VirR, respectively. (C) Lane 1, no-VirR control; lane 2, target DNA incubated with 1 µg of VirR. (D) Lanes 1 and 2, 278-bp fragment incubated with no protein or 1 µg of VirR, respectively. Shifted bands are indicated by the arrows.

A 393-bp fragment (from $-$ 252 to +142 with respect to the transcription start site) containing the single plc promoter (3),as well as a regulatory deoxyribosyladenine rich region that isinvolved in DNA bending (30, 57), was used as the target DNAin gel mobility shift experiments. The results showed that whenthis DNA target was incubated with different amounts of VirR,no shifts in DNA mobility were observed (Fig. 2A).

In contrast to what was found for the plc gene, two promoters have been identified upstream of the colA gene (3). Basedon primer extension analysis, the promoter closer to the startof the gene, P₂, was found to be virRS dependent, while the promoterlocated further upstream, P₁, was found to be virRS independent(3). Therefore, initially a 304-bp fragment ( $-$ 136 to +169)containing the P₂ promoter was amplified, labelled, and used asthe DNA target. Once more the results showed that VirR did notbind to this region, since no shifts in DNA mobility were observedwhen the target fragment was incubated with VirR (Fig. 2B).

The pfoR gene is located immediately upstream of pfoA (49). Since the pfoR promoter has not been identified, a 408-bp DNAfragment that encompassed the start of pfoR and 327 bp of sequencelocated upstream of the ATG start codon was used as the target(Fig. 2C). Like that of the regions upstream of the plc and colAgenes, the mobility of the pfoR upstream regions did not shiftin the presence of VirR (Fig. 2C). Based on these data it wasconcluded that VirR does not bind to the regions immediately upstreamof the plc, colA, and pfoR genes. Note that with all of the targetDNA fragments, the gel shift experiments were repeated in thepresence of 50 mM acetyl phosphate. The same results were obtainedin the presence of this low-molecular-weight phosphodonor (datanotshown).

The final region of interest was upstream of the pfoA gene, which is transcribed from a major virRS-dependent promoter. Thisregion was divided into two target fragments, a 211-bp fragment(+176 to +387) that contained two inverted repeats and a 278-bpregion ( $-$ 99 to +180) that contained a cluster of direct repeatsas well as the pfoA promoter. When the 211-bp fragment was incubatedwith VirR, its mobility was found to be unaltered (Fig. 3C), providingevidence that VirR does not bind to the inverted repeats. However,when the 278-bp fragment was incubated with VirR, two bands ofaltered mobility were observed (Fig. 2D). This experiment providedthe first evidence that VirR had the ability to bind to a regionlocated directly upstream of one of its targetgenes.

To further localize the VirR binding site and to determine whether the regulatory protein was bound to the cluster of directrepeats or to the region surrounding the promoter, the 278-bpfragment was divided into two separate, slightly overlapping targetfragments, a 114-bp fragment (+66 to +180) that contained thedirect repeats and a 183-bp fragment ( $-$ 99 to +85) that encompassedthe promoter region (Fig. 3). When these fragments were incubatedwith 1 or 2 µg of VirR, only the fragment containing the pfoApromoter had an altered electrophoretic mobility (Fig. 3A andB). As previously observed with the 278-bp fragment, two bandsof altered mobility were observed. These bands were designatedcomplex I (CI) and complex II (CII) (Fig. 3). These experimentsdemonstrated that VirR could bind to the promoter region of pfoA.Furthermore, this binding was shown to be specific, since theaddition of various amounts of unlabelled 183-bp DNA fragmentgradually reduced the amount of the CII band, and, to a lesserextent, the CI band (Fig. 4A). In addition, binding specificitywas demonstrated by the lack of inhibition by a nonspecific competitor(the unlabelled 408-bp pfoR upstream region) when added at thesame concentration as that of the specific competitor (Fig. 4A).Binding to the 183-bp fragment was dependent upon the concentrationof VirR, since increasing the amount of VirR in the binding assaymixture progressively led to an increase in the amount of CI andCII, with a concomitant decrease in the amount of free unboundtarget DNA (Fig. 4B). As before, the addition of acetyl phosphatedid not have any effect on the binding of the protein; that is,incubation in the presence of acetyl phosphate did not increasethe VirR binding affinity.

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FIG. 3. Gel shift analysis of the pfoA gene region. The pfoA-derived DNA fragments used in the gel mobility shift assays (bars) and their respective sizes (in base pairs) are shown. The direct repeats in the 114-bp fragment, the promoter in the 183-bp fragment, and the inverted repeats in the 211-bp fragment, are shown as directly repeated arrows, a bent arrow (P_pfoA), and inverted arrows, respectively. (A and B) Lane 1, no-VirR control; lanes 2 and 3, DIG-labelled DNA incubated with 1 and 2 µg of VirR, respectively. The VirR-DNA complexes CI and CII are indicated. (C) Lane 1, no-VirR control; lane 2, DIG-labelled fragment incubated with 1 µg of VirR. (D) Lane 1, no-VirR control; lanes 2 to 5, target DNA incubated with 1 µg of VirR. Reaction mixtures in lanes 3 to 5 also contained 15 pmol of the following unlabelled fragments: lane 3, 302-bp fragment (specific competitor); lane 4, 183-bp of unlabelled upstream pfoA fragment; lane 5, 408-bp upstream pfoR fragment (nonspecific competitor).

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FIG. 4. Specificity and VirR dependence of DNA binding. (A) Competitive binding gel shift assay. The DIG-labelled 183-bp pfoA fragment was incubated with 1 µg of VirR and various amounts of unlabelled 183-bp DNA (specific competitor). Lane 1, no-VirR control; lanes 2 to 6, target DNA that was incubated with 1 µg of VirR. These incubation mixtures also contained 0, 3.0, 7.5, 15, and 30 pmol of specific competitor DNA, respectively. Lane 7, DIG-labelled DNA incubated with 1 µg of VirR and 30 pmol of nonspecific competitor (408-bp upstream pfoR fragment). (B) Concentration dependence of VirR binding. The [ $alpha$ -³²P]dATP-labelled 183-bp pfoA fragment was incubated with various amounts of VirR and examined by gel shift analysis as described above except that the data were obtained and quantitated in a phosphorimager. The amount of labelled DNA in each band was calculated and plotted as shown. The amounts of free DNA (F), CI complex, CII complex, and total complex (CI+CII) are shown.

Binding of VirR was also detected with an internal 302-bp pfoA region (+436 to +737) (Fig. 3D, lane 2). However, the bindingwas weaker and was found to be nonspecific, since the additionof a specific competitor (the same unlabelled fragment) (Fig.3D, lane 3) gave a binding profile similar to that obtained inthe presence of the nonspecific competitor (the 408-bp upstreampfoR fragment) (Fig. 3D, lane 5). Furthermore, when the unlabelled183-bp pfoA fragment was added at the same concentration, theshifted band was no longer observed (Fig. 3D, lane 4). Similarnonspecific binding was also found with the 383-bp internal plcgene region (+251 to +634), the 348-bp internal colA gene region(+150 to +397), the 402-bp internal pfoR gene region, and the275-bp region ( $-$ 389 to $-$ 117) encompassing the VirR-independentcolA promoter, P₁ (data not shown). The locations of these fragmentsare shown in Fig. 2. Once more, the addition of acetyl phosphateto these binding reaction mixtures did not have any effect onVirRbinding.

Identification of the VirR binding site. To identify the VirR binding site, DNase I footprinting was carried out on both sense and antisense strands. The 257-bp DNAtarget, which encompassed the pfoA promoter region, was obtainedby PCR from pJIR1546 (Table 1) with primers 6519 and 5126. Inseparate PCR experiments, one primer was labelled with [ $gamma$ -³²P]ATP so that only one DNA strand was end-labelled. When theselabelled DNA fragments were incubated separately with VirR andthen partially digested with DNase I, a protected region was observedon both DNA strands (Fig. 5A and B). Comparison with a DNA sequencingladder revealed that the region of protection on both strandsoverlapped and was located immediately upstream of the pfoA promoter(Fig. 6A). The region of overlap was termed the core binding regionand was found to be approximately 52 bp in length.

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FIG. 5. DNase I footprinting analysis. Results of footprinting reactions where either the sense or antisense DNA strands were labelled with [ $gamma$ -³²P]ATP are shown. Sequencing reactions with the same oligonucleotide primers used to generate the PCR products are shown next to the footprinting reactions. The $-$ 10 and $-$ 35 boxes are represented by the black rectangles. (A and B) Identification of the VirR binding site. Regions protected from DNase I digestion are represented by the open rectangles. The transcription start point is shown as +1, and the positions of the regions of protection relative to +1 are as indicated. (C and D) Analysis of the VirR binding site deletion derivative. The site of deletion is indicated by the asterisk. In all panels, lane 1 contains no VirR and lanes 2 and 3 contain 1 and 2 µg of VirR, respectively. All footprinting reaction mixtures contained 25,000 cpm of labelled DNA.

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FIG. 6. Sequence and mutations of the VirR binding site. (A) Sequence of the core binding region site (boldface). The imperfect direct repeats within this region are indicated by the dashed arrows. The nucleotide residues that were changed by site-directed mutagenesis are shown above the original nucleotide sequence. The $-$ 35 and $-$ 10 boxes of the pfoA promoter are underlined, the transcriptional start point (tsp) is indicated by the bent arrow, and the start of the pfoA gene is indicated by the solid arrow. The 49-bp region deleted by SOE PCR is shown as the gray rectangle. (B) Gel mobility shift assays carried out on the deletion derivatives. Lane 1, wild-type 183-bp fragment incubated with 1 µg of VirR; lanes 2 and 3, 134-bp deletion fragment incubated with either no VirR or 1 µg of VirR, respectively. (C) Gel mobility shift assay with direct repeat mutation derivatives. The imperfect direct repeats were altered by site-directed mutagenesis. Lanes 1 and 2, DNA fragment with intact direct repeats; lanes 3 to 5, DNA fragments with mutations in DR1, DR2, or DR1 and DR2, respectively. All binding reaction mixtures contained 1 µg of VirR, with the exception of the no-protein control in lane 1.

To confirm that this region was required for VirR binding, 49 bp of the 52-bp core binding region was deleted by SOE PCR.The resultant PCR product was then labelled with DIG and usedas the target DNA in gel mobility shift experiments. The resultsshowed that when this region was deleted, no DNA mobility shiftwas observed in the presence of purified VirR (Fig. 6B). Theseobservations were confirmed by DNase I footprinting. When thecore binding region was removed, the DNA footprint was no longerobserved after incubation with VirR (Fig. 5C and D). These dataprovided clear evidence that the core binding region identifiedby DNase I footprinting was essential for the binding of VirRto the pfoA promoterregion.

VirR binds to directly repeated sequences located immediately upstream of the pfoA promoter. In other two-component signal transduction systems, the response regulators have been shown to bind to direct or invertedrepeats located in the promoter region (16, 33). Previousnucleotide sequence analysis of the pfoA upstream region revealedthe presence of two imperfect direct repeats (CCCAGTTNTNCAC) immediatelyupstream of the $-$ 35 box of the pfoA promoter (3). These repeats,which we have designated DR1 and DR2 (Fig. 6A), were located inthe core binding region and are different from those in the 114-bpDNA fragment. Therefore, to determine whether DR1 or DR2 or bothwere directly involved in VirR binding, the repeats were alteredby site-directed mutagenesis. In these experiments, the CCA residuesof bases 2 to 4 of the direct repeats in the target plasmid, pJIR1546(Table 1), were changed to TAG either individually to producepJIR1804 (DR1 altered) and pJIR1803 (DR2 altered) or togetherto construct pJIR1821 (both DR1 and DR2 mutated) (Fig. 6A). Eachaltered insert was completely resequenced to confirm that no othermutations had been introduced. The 183-bp DNA fragments from pJIR1546and its mutated derivatives were then amplified and analyzed fortheir abilities to bind VirR in gel mobility shift assays. Theresults showed that when either DR1 or DR2 was altered, VirR couldbind to the target DNA to form CI but that very little CII wasobserved (Fig. 6C). However, when both DR1 and DR2 were mutated,VirR binding was almost eliminated, as no CII was observed andonly a very faint CI band was evident (Fig. 6C). These resultsclearly demonstrated that the CCA residues in the direct repeatswere required for VirRbinding.

To determine if VirR bound to only the wild-type sites in the mutated regions or bound to both sites but was no longer ableto form a second-stage complex, DNase I footprinting studies werecarried out. For each plasmid derivative the sense DNA stand wasend-labelled with [ $gamma$ -³²P]ATP, incubated with VirR, and then partially digested with DNaseI. When both direct repeats were intact (pJIR1546 template), thenormal footprint was observed (Fig. 7, lane 2). When DR1 was mutated,a region of DNA protection was observed in the DR2 region, butno footprint was observed in the DR1 region (Fig. 7, lane 4).The DNase I digestion profile in this area was the same as thatfor the corresponding region in the no-protein control (Fig. 7,lane 3). Similarly, when DR2 was mutated, a DNA footprint wasobserved in the DR1 region but no DR2 footprint was evident (Fig.7, lane 6). Again the digestion profile was the same as that forthe corresponding area in the no-VirR control (Fig. 7, lane 5).Finally, when both repeats were mutated, no footprints were detectedin either region (Fig. 7, lane 8). Based on these data it wasconcluded that the direct repeats constituted two individual VirRbinding sites. Furthermore, binding to these sites was not cooperative,since mutation of one site did not eliminate binding to the othersite.

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FIG. 7. DNase I footprinting analysis of direct-repeat mutants. The labelled plasmid templates used in this experiment were the wild-type plasmid pJIR1546 (lanes 1 and 2) and the mutated derivatives pJIR1804 (DR1 mutant; lanes 3 and 4), pJIR1803 (DR2 mutant; lanes 5 and 6), and pJIR1821 (DR1-DR2 double mutant; lanes 7 and 8). Lanes 1, 3, 5, and 7, control reaction mixtures that were not preincubated with VirR. Lanes 2, 4, 6, and 8, test reaction mixtures that were incubated with 2 µg of VirR prior to partial digestion by DNase I and electrophoresis. The first four lanes (ACGT) show the sequencing reaction products from the wild-type pJIR1546 template. Lanes 9 to 11, C track sequencing reaction products from pJIR1804, pJIR1803, and pJIR1821, respectively. The positions of the DR1 and DR2 repeats are shown by the arrows, and the region of protection is represented by the open rectangle. The $-$ 10 and $-$ 35 boxes are depicted as black rectangles, and the transcription start point is shown as +1.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Most response regulators consist of a conserved N-terminal receiver domain and a unique C-terminal domain that interacts withthe target genes. These proteins may be divided into differentsubclasses according to the nature of their C-terminal domains(1). Many response regulators contain a helix-turn-helix DNAbinding motif in this region (1, 38), although others, suchas OmpR, have a helix-loop-helix or winged-helix domain (29,34). In C. perfringens, the VirR response regulator is responsiblefor the transcriptional activation of genes involved in toxinproduction. These genes include the plc, colA, and pfoA genes(27, 48). The N-terminal region of VirR has significant aminoacid sequence similarity to those of other response regulators,in particular the conserved residues involved in phosphorylation(27). However, no helix-turn-helix motif has been identifiedin the C-terminal domain of VirR. In addition, upstream of theplc, colA, and pfoA genes, no common sequences which could actas conserved DNA binding motifs have been identified (3). Therefore,it was possible that VirR did not bind to a single consensus sitebut to various regions located upstream of the different targetgenes. Alternatively, VirR may regulate transcription of one ormore of the target genes by activating the transcription of genesthat encode other, as yet unidentified, regulatoryproteins.

In this study, a His-tagged VirR protein was purified and subsequently tested in gel mobility shift assays for its abilityto bind to the various promoter regions of the plc, colA, pfoR,and pfoA genes. VirR was found to only bind specifically to thepfoA promoter region, producing two complexes of altered electrophoreticmobilities. This result is consistent with the previously observeddifferential effects of mutation of the chromosomal virR (48)and virS (27) genes. These mutants produce reduced but detectiblelevels of alpha-toxin and collagenase. However, they do not haveany detectible perfringolysin O activity, suggesting that thepfoA gene is regulated in a different manner from the other targetgenes (27, 48). Subsequent transcriptional analysis was inaccordance with the observed toxin phenotypes, and it was suggestedthat expression of the plc, colA, and pfoR genes involves otherregulatory genes in addition to the virS/virR system (3). Ourresults are in agreement with this hypothesis as they show thatVirR does not bind to the promoter regions of thesegenes.

Previous studies indicated that the product of the pfoR gene, which is located approximately 500-bp upstream of pfoA, activatedthe expression of pfoA in E. coli (49). It was subsequentlypostulated that VirR may activate the transcription of pfoA indirectlyby regulating the expression of the pfoR gene (3). In suchcircumstances VirR would not bind to the pfoA gene region. However,our results provide strong evidence that VirR acts directly onthe pfoA promoter rather than through a regulatory cascade involvingPfoR. These data do not rule out the possibility that PfoR mayalso regulate pfoA expression. Resolution of the role of PfoRawaits the construction and analysis of chromosomal pfoR mutantsin C. perfringens.

DNase I footprinting and deletion analysis showed that VirR bound to a core 52-bp sequence located immediately upstream ofthe $-$ 35 region of the pfoA promoter. Many response regulatorshave been shown to bind in close proximity to the $-$ 35 boxes oftheir target gene promoters and to regulate transcription by modulatingthe binding of RNA polymerase to the promoter. Interaction betweenresponse regulators such as BvgA from Bordetella pertussis (6,7), PhoP from Bacillus subtilis (42), and PhoB from E. coli(28) and their respective RNA polymerase has been demonstrated.We postulate that VirR activates pfoA transcription by eitherfacilitating the binding of RNA polymerase to the promoter orby altering the conformation of the polymerase-promoter complexso that transcription can occur. Therefore, in the absence ofVirR either RNA polymerase cannot bind to the promoter or it bindsbut cannot initiate transcription. In both situations no perfringolysinO isproduced.

Sequence analysis of the VirR binding site revealed the presence of two CCCAGTTNTNCAC imperfect direct repeats (3). Theserepeats are not found in any of the other target gene regions.Many well-studied response regulators such as PhoP (12, 24,25) and OmpR from E. coli (15, 41) have been shown to bindto short directly repeated sequences. Gel shift analysis of site-directedmutants of the pfoA repeats indicated that they were requiredfor VirR binding. Mutation of either repeat almost eliminatedthe formation of the less-mobile CII VirR-DNA complex and significantlyreduced the affinity of VirR for the DNA binding site, as observedpreviously with AlgR from Pseudomonas aeruginosa (36). Mutationof both repeats virtually eliminated VirR binding, providing directevidence that VirR requires the CCA nucleotides of the repeatsequences forbinding.

These results can be explained by postulating that the repeats represent two separate VirR binding sites, whereby CI representsa VirR-target DNA complex at either binding site and CII resultsfrom VirR binding at both sites. Alternatively, binding may havebeen cooperative, with both sites being required for VirR binding.However, DNase I footprinting of the site-directed mutants providedstrong evidence that the direct repeats represented two separateVirR binding sites. When either repeat was mutated, only the footprintprotecting the remaining wild-type repeat was observed. That is,the alteration of one repeat did not appear to affect the abilityof VirR to bind to the other repeat. If binding was cooperative,mutation of one direct repeat would most likely reduce the abilityof VirR to bind to the other binding site, as observed with NtrCfrom E. coli (9, 59), or prevent the binding of VirR to thewild-type site, as observed with PhoP (25).

In addition to the specific binding observed with the 183-bp pfoA fragment, several internal gene regions were also foundto bind VirR, albeit nonspecifically. This interaction most likelyrepresents genuine nonspecific binding. Sequence alignments ofthese regions did not show any regions of conservation, nor werethere any similarities to the pfoA VirR binding region. The bindingof response regulators to internal gene regions has recently beenobserved with genes regulated by the PhoP/PhoR system in B. subtilis(25). However, these regions were found to contain the consensusbinding sequence. It is possible that although binding to thepfoA region is sequence specific, as demonstrated by the mutationalanalysis, the nonspecific binding to the internal gene regionsmay be due to secondary structure similarities. Alternatively,the nonspecific binding may be due to the absence of a bindingcofactor such as RNA polymerase. The synergistic binding of RNApolymerase and the BvgA response regulator has been observed (6,7). Important interactions between the $alpha$ -subunit of RNA polymeraseand OmpR have also been observed (47, 51). Future studieswill need to involve an examination of the possible interactionsbetween C. perfringens RNA polymerase andVirR.

With most response regulators, phosphorylation plays a key role in protein function. In most systems, phosphorylation canincrease the binding affinity for the target DNA so that the regulatoryprotein can bind to secondary lower-affinity binding sites (6,8, 16, 25), alter the DNA binding pattern (10), or initiatecooperative binding (9, 18, 59). However, some responseregulators are able to bind when not phosphorylated, albeit withlower affinity (16, 23, 28, 42). The observation thatthe addition of acetyl phosphate did not alter the gel shift resultssuggested that DNA binding was not dependent on phosphorylation.One possible explanation for this result is that the VirR moleculesmay already be at least partially phosphorylated by sensor kinasecross talk or by low-molecular-weight phosphodonors present inthe expression host cells. Nonspecific phosphorylation of responseregulators does occur in other systems (40). However, it seemsunlikely that the VirR protein phosphorylated by such mechanismswould remain in the active phosphorylated state during longer-termstorage of the purified protein. Note that we cannot rule outthe possibility that although acetyl phosphate did not affectVirR binding, other low-molecular-weight phosphodonors may havedemonstrableeffects.

While acetyl phosphate is often used as the phosphodonor for many response regulators, it is possible that this phosphodonordoes not phosphorylate VirR or does so inefficiently. Either way,the addition of acetyl phosphate would have little or no observableeffect. Different reactivities toward various phosphodonors havebeen previously demonstrated by several response regulators. CheYcan be phosphorylated by acetyl phosphate, carbamoyl phosphate,and phosphoramidate (26), while phosphoramidate is used exclusivelyby CheB (26) and preferentially by NRI (or NtrC) (32). Therefore,further work is required to test for phosphorylation of VirR byotherphosphodonors.

A more plausible explanation is that phosphorylation of the response regulator is not required for in vitro binding to thespecific pfoA target site. Even though phosphorylation may berequired in vivo for VirR binding, it may not be required at theVirR concentrations used in the in vitro binding experiments.BvgA (5) and PhoB (28) can still bind DNA when the N-terminalregion, which is essential for phosphorylation, has been removed.However, phosphorylation is required for transcriptional activation(5, 28, 42). More specifically, it is the phosphorylatedresponse regulator that interacts with RNA polymerase, which inturn leads to gene transcription. Therefore, it is also possiblethat phosphorylation of VirR is required for transcriptional activationbut not for DNAbinding.

Based on the data presented in this paper we have modified the previous model (50) for the regulation of toxin productionin C. perfringens (Fig. 8). We propose that when VirS detectsan environmental or growth phase stimulus, it autophosphorylatesat H255. Phosphorylated VirS is then able to donate the phosphorylgroup to VirR, which is phosphorylated at D57. Once activated,VirR binds upstream of the pfoA promoter and activates the transcriptionof pfoA so that perfringolysin O is produced. Transcription ofpfoA is VirR dependent, to the extent that no perfringolysin Ois produced in the absence of a functional virRS operon. In addition,pfoA expression may also be controlled by another regulatory protein,PfoR (49). It also appears that VirR acts in conjunction withother regulatory factors to activate the transcription of theplc and colA genes so that increased levels of alpha-toxin andcollagenase are produced (3). Although we have now shown thatVirR binds directly to the pfoA promoter region there are stillmany aspects of the VirS/VirR two-component signal transductionsystem that are yet to be elucidated. These features include thenature of the external stimulus that activates VirS, the natureof the other putative regulatory genes that may be involved inthe regulatory cascade, the extent of the regulatory network,and, most importantly, the effect of the mutated direct repeatson pfoA expression in vivo. However, it is hoped we are now atleast one step closer to the elucidation of the overall mechanismby which toxin production and virulence are regulated in C. perfringens.

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FIG. 8. Proposed model of the VirS/VirR two-component signal transduction system. The genes postulated to be controlled by the VirS/VirR network are shown as light gray boxes. The dark gray rectangles represent the VirS sensor histidine kinase, while the VirR response regulator is depicted by the dark gray ovals. The presence of other activator(s) is symbolized by the black oval. The unknown protease and sialidase genes are represented by prt and nan, respectively.

	ACKNOWLEDGMENTS

This research was supported by grants from the Australian National Health and Medical Research Council. J.K.C. was the recipientof an Australian PostgraduateAward.

We thank Rocco Iannello and Julia Young for helpful advice anddiscussions.

	FOOTNOTES

^* Corresponding author. Mailing address: Bacterial Pathogenesis Research Group, Department of Microbiology, Monash University,Clayton 3800, Australia. Phone: 61 3 9905 4825. Fax: 61 3 99054811. E-mail: Julian.Rood{at}med.monash.edu.au.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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