The Pseudomonas aeruginosa Exotoxin A Regulatory Gene, ptxS: Evidence for Negative Autoregulation

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Journal of Bacteriology, August 1999, p. 4890-4895, Vol. 181, No. 16
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

The Pseudomonas aeruginosa Exotoxin A Regulatory Gene, ptxS: Evidence for Negative Autoregulation

Britta L. Swanson, Jane A. Colmer, and Abdul N. Hamood^*

Department of Microbiology and Immunology, Texas Tech University Health Sciences Center, Lubbock, Texas 79430

Received 30 March 1999/Accepted 9 June 1999

	ABSTRACT

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We have previously described a Pseudomonas aeruginosa gene, ptxR, which enhances exotoxin A production at the transcriptionallevel. We have also described another gene, ptxS, which is transcribeddivergently from ptxR and interferes with the enhancement of exotoxinA synthesis by ptxR. However, the mechanisms through which ptxRand/or ptxS are regulated is not known. In this study, we attempted(by using the DNA gel shift assay) to determine if P. aeruginosacontains a potential regulatory protein that binds specificallyto the ptxR or ptxS upstream region. In the initial analysis,different-sized gel shift bands were detected when a probe containingthe ptxR-ptxS intergenic region was incubated with the lysateof P. aeruginosa PAO1. The strongest binding activity was detectedwith a smaller fragment that represents the ptxS upstream region.Additional deletion analysis localized the binding to a 52-bpfragment immediately upstream of ptxS. The gel shift band wasnot detected when the 52-bp fragment was incubated with the lysateof the ptxS isogenic mutant PAO1::ptxS. However, the binding bandwas regenerated when a plasmid carrying ptxS intact was introducedinto PAO1::ptxS. In addition, the gel shift band was detectedwhen the 52-bp fragment was incubated with a lysate of Escherichiacoli in which ptxS was overexpressed from the T7 promoter. Theeffect of PtxS on ptxS expression was examined by using a ptxS-lacZfusion plasmid. The level of $beta$ -galactosidase activity producedby PAO1::ptxS carrying the fusion plasmid was four- to fivefoldhigher than that produced by PAO1 carrying the same plasmid. UsingDNase I footprinting analysis, the binding region was specifiedto a 20-bp fragment. Within the fragment, a 14-bp palindromicsequence exists that may function as a PtxS binding site. Theseresults suggest that PtxS autoregulates its synthesis by bindingto a specific sequence within the ptxS upstreamregion.

	INTRODUCTION

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Pseudomonas aeruginosa is a gram-negative pathogen that causes a variety of infections, including wound infections, nosocomialinfections, and lung infections in cystic fibrosis patients (3,34). The ability of P. aeruginosa to cause these infectionsis due to the production of several extracellular virulence factors(35). Among these different virulence factors, exotoxin A isconsidered the most toxic. Exotoxin A is an ADP-ribosyltransferaseenzyme that catalyzes the transfer of the ADP-ribosyl moiety ofNAD⁺ onto elongation factor 2 of eukaryotic cells, causing cessationof the protein synthesis process and subsequent cell death (12).In vitro production of exotoxin A by P. aeruginosa is controlledby different environmental factors. These factors include thelevel of iron in the growth medium, the growth temperature, andthe presence of certain amino acids and nucleotides in the growthmedium (2, 13).

Exotoxin A production by P. aeruginosa is a complicated process that involves several positive and negative regulatory genes(7, 19, 31, 33). One of the most extensively analyzedof these genes is regA, which is required for maximum productionof exotoxin A by P. aeruginosa (33). A P. aeruginosa mutantdefective in regA produces neither regA nor toxA mRNA (24, 33).The regA gene, which codes for a 28-kDa protein, enhances exotoxinA production at the transcriptional level (33). We have previouslydescribed another toxA regulatory gene, ptxR (9). The presenceof a plasmid carrying ptxR in P. aeruginosa enhances exotoxinA production four- to fivefold (9). The ptxR gene encodes a34-kDa protein that belongs to the LysR family of transcriptionalactivators and enhances toxA transcription through regA (9).However, the exact mechanism of this regulation is still unknown.In addition to exotoxin A, ptxR positively regulates the productionof the P. aeruginosa siderophores pyochelin and pyoverdine (6).However, the mechanism of this regulation appears to be differentfrom that of exotoxin A. Although ptxR enhances exotoxin A productionin P. aeruginosa, it does not interfere with the negative regulationof exotoxin A synthesis by iron (9). In contrast, siderophoreproduction in P. aeruginosa carrying a ptxR plasmid is deregulatedwith respect to iron (6).

We have recently described another toxA regulatory gene, ptxS, which interferes with the effect of ptxR on toxA transcription(6). The product of ptxS, PtxS, is a 37-kDa protein which belongsto the GalR family of transcriptional repressors (6). Althoughthe exact mechanism of PtxS function is not known, available evidencesuggests that ptxS negatively regulates the transcription of ptxR(6). The ptxS gene, which is located 5' of ptxR, is transcribedin the opposite orientation of ptxR (6). Between the ptxR andptxS translational start codons is a 562-bp intergenic region(6). Despite the analysis of ptxR and ptxS functions, the mechanismsthrough which these genes are regulated are unknown. In this study,we attempted to determine if P. aeruginosa contains a proteinthat specifically binds to either the ptxR or the ptxS upstreamregion (a potential DNA binding regulatory protein). Our resultsshowed that PtxS negatively autoregulates its own synthesis bybinding specifically to the ptxS upstreamregion.

	MATERIALS AND METHODS

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Bacterial strains, plasmids, media, and growth conditions. The bacterial strains and plasmids used in this study are listed in Table 1. Escherichia coli strains were grown in Luria-Bertanimedium (1% Bacto Tryptone [Difco Laboratories, Detroit, Mich.],0.5% yeast extract, 1% NaCl). For binding experiments, P. aeruginosawas grown in Chelex-treated Trypticase soy broth dialysate (BBLMicrobiology Systems, Cockeysville, Md.) to which 1% glyceroland 0.05 M monosodium glutamate were added (TSB-DC) (17). Cultureswere grown at 37°C with vigorous aeration. Antibiotics were usedat the following concentrations: ampicillin, 75 µg/ml (E. coli);carbenicillin, 100 (E. coli) or 300 (P. aeruginosa) µg/ml; rifampin,80 µg/ml (P. aeruginosa).

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TABLE 1. Bacterial strains and plasmids used in this study

Preparation of cell extracts. P. aeruginosa PAO1 was grown in 100 ml of TSB-DC at 30°C for 14 h. The cells were harvested, resuspended in 10 ml of distilledwater (10× concentration), and lysed by being passed twice througha French pressure cell at 1,000 lb/in² (American Instrument Company, Silver Spring, Md.). Lysed cellswere centrifuged at 240 × g, and the supernatant fraction (whichrepresents the cell lysate) was isolated and divided into severalaliquots. The amount of protein in each sample was determinedby the method of Lowry et al. (14).

Gel shift assay. DNA fragments containing different segments of the ptxS upstream region were obtained by either restriction digestions orPCR (32). The fragments were labeled with [ $gamma$ -³²P]ATP (Amersham, Arlington Heights, Ill.) by the end-labelingtechnique using T4 polynucleotide kinase (1). The binding experimentswere performed as previously described (1). The binding reactionmixture (20-µl total volume) contained DNA binding buffer (10mM Tris-HCl [pH 7.4], 1 mM EDTA, 10 mM KCl, 0.1 mM dithiothreitol,5% glycerol, 50 µg of bovine serum albumin per ml), 1 µg of poly(dI-dC)(Boehringer Mannheim, Indianapolis, Ind.) per ml (for nonspecificbinding), and 25 to 50 µg of the 10× PAO1 lysate. Approximately10⁷ cpm of radiolabeled DNA probe was added, and the reaction mixturewas incubated at 30°C for 30 min. Approximately 3 µl of the trackingdye (50% sucrose, 0.6% bromphenol blue) was added to the reactionmixture, and it was loaded onto an 8% polyacrylamide gel in 1×Tris-borate-EDTA buffer (1). The gel was electrophoresed at180 V for 2.5 h. The gels were dried and exposed to X-rayfilm.

DNase I footprint analysis. The 103-bp fragment which corresponds to the ptxS upstream region was synthesized by PCR. The fragment was end labeled byusing T4 polynucleotide kinase (1). One label was then removedby using the KpnI restriction enzyme. The singly labeled DNA fragmentwas incubated with 5 to 25 µg of the partially purified proteinby using a reaction mixture identical to that described abovefor the gel shift assay. After 30 min of incubation at 30°C, thereaction mixture was manipulated as listed in the manufacturer'sinstructions (Core Footprinting System; Promega, Madison, Wis.).Fifty microliters of a Ca²⁺-Mg²⁺ solution was added, and the mixture was incubated for 1 min atroom temperature; approximately 3.5 × 10² U of DNase I was added, and the mixture was incubated for 1 minat room temperature; and the reaction was stopped by the additionof 75 µl of the Stop Solution supplied in the footprinting kit.The reaction was phenol extracted and precipitated in ethanol.The DNA was resuspended in loading buffer and separated on a 10%sequencinggel.

Construction of pBS8-4. The 740-bp BamHI/ScaI fragment containing 726 bp of the ptxS upstream region and 14 bp of the ptxS structural gene was isolatedfrom pJAC13 (6). The 3' and 5' ends were converted to bluntends, and the fragment was cloned into the SmaI site of pUC18.The ptxS upstream region was then isolated from the resultingrecombinant plasmid as a BamHI/EcoRI fragment. The 5' ends wereconverted to blunt ends, and the fragment was cloned in the SmaIsite of the lacZ translational fusion vector pSW205 (23). Throughthese different manipulations, a 7-bp pUC18 sequence was addedto the 14 bp of the ptxS structural gene. Nucleotide sequenceanalysis was performed to confirm the construction of pBS8-4.

Enzyme assay. Levels of $beta$ -galactosidase activity were determined as previously described (16). A 1-ml pellet was washed and resuspendedin 100 µl of distilled water, and the membranes were disruptedby sonication. Statistical analysis was done by the paired t test(22) using the computer program InStat 2.01 (GraphPad Software,San Diego, Calif.).

Expression experiments. PtxS was overproduced in E. coli K38 by using the T7 expression system as previously described (6, 26).

	RESULTS

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Identification of the potential DNA binding protein. Despite our previous analysis of the P. aeruginosa ptxR gene, its effect on the expression of the toxA and regA genes, andthe interaction between the ptxR and ptxS genes, we still do notknow the factors or the specific conditions that regulate theexpression of either gene. One possible mechanism for such regulationis through transcriptional factors (positive or negative) thatspecifically bind to the upstream region of ptxR, ptxS, or both.Computer analysis revealed that the ptxR and ptxS upstream regionscontain specific sequences that may represent binding sites forregulatory proteins (6). Therefore, we have utilized the DNAgel shift assay to determine if P. aeruginosa contains a protein(s)that specifically binds to the ptxS or ptxR upstream region. Thesource of the putative protein was the lysate of P. aeruginosaPAO1 (both ptxR and ptxS were originally isolated from PAO1) thatwas grown in an iron-deficient medium (TSB-DC). The probe forinitial gel shift experiments was the 740-bp BamHI-KpnI fragmentcontaining 553 bp of the ptxR-ptxS intergenic region (ptxR andptxS are divergently transcribed) (6) and 167 bp of the ptxRstructural gene (Fig. 1). Two gel shift bands were detected whenthe P. aeruginosa lysate was incubated with the 740-bp fragment(data not shown). Since this intergenic fragment contains boththe ptxS and ptxR upstream regions, we attempted to assign theobserved binding to either the ptxR or the ptxS upstream regionby dividing the fragment. The 740-bp fragment was divided intothree smaller fragments by using available restriction sites:a 257-bp BamHI-DpnI fragment containing the putative upstreamregion of ptxR and a portion of its open reading frame, a 157-bpDpnI-DpnI intergenic fragment, and a 304-bp DpnI-KpnI fragmentcontaining the putative upstream region of ptxS (Fig. 1). Twogel shift bands with strong intensity were detected when the 304-bpprobe was incubated with the PAO1 lysate (25). A fainter gelshift band was detected when the 157-bp probe was incubated withthe PAO1 lysate (25). Since the binding to the 304-bp probewas consistently detected and remained very intense, further experimentswere conducted focusing on the localization and purification ofthe potential DNA binding protein(s). Additional subcloning andgel shift experiments further found that the binding activitycould be assigned to two separate DNA regions: a 201-bp fragmentand a 103-bp fragment (25; Fig. 2A). Since the 103-bp fragmentwas located immediately upstream of ptxS and represented a putativeptxS regulatory region, we chose to focus on the purificationof this potential DNA binding protein and define the specificsequence to which it binds. The 103-bp fragment was subsequentlydivided into two smaller fragments: a 52-bp fragment and a 63-bpfragment (Fig. 1). Since no suitable restriction sites were availableto generate these two fragments, they were synthesized by PCR.A gel shift band was detected with the 52-bp fragment only (Fig.2A). The binding specificity was confirmed by competition experimentsusing the 103-bp probe and the unlabeled 52- or 63-bp fragment.Only when an excess of the unlabeled 52-bp fragment was addedto the binding reaction mixture (103-bp probe and PAO1 lysate)did the binding band disappear (Fig. 2B). These results suggestthat the PAO1 lysate contains a potential DNA binding proteinthat specifically binds to the ptxS upstream region.

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FIG. 1. Diagram of the different probes (within the ptxR-ptxS intergenic region) that were used in the gel shift assays. The 304- and 103-bp fragments of the ptxS upstream region were generated by restriction digestion using available restriction sites (B, BamHI; D, DpnI; H, HincII; K, KpnI). The 52- and 63-bp fragments were synthesized by PCR. Arrows indicate the direction of transcription of ptxR and ptxS.

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FIG. 2. (A) Electrophoretic mobility shift assay of three different probes incubated with the lysate of P. aeruginosa PAO1. The binding reaction mixtures are described in Materials and Methods. Each DNA-protein reaction mixture contained 25 µg of the PAO1 lysate. F, free probe; C, DNA-protein complex. Lanes: 1, 103-bp probe alone; 2, 103-bp probe plus PAO1 lysate; 3, 52-bp probe alone; 4, 52-bp probe plus PAO1 lysate; 5, 63-bp probe alone; 6, 63-bp probe plus PAO1 lysate. (B) Competitive gel shift assay using the labeled 103-bp probe and the unlabeled 52- or 63-bp fragment. The DNA-protein binding reaction mixtures contained 25 µg of PAO1 lysate. Lanes: 1, 103-bp probe alone; 2, 103-bp probe plus PAO1 lysate plus 52-bp fragment; 3, 103-bp probe plus PAO1 lysate plus 63-bp fragment; 4, 103-bp probe plus PAO1 lysate (control).

Binding of PtxS to the ptxS upstream region. Homology searches showed that PtxS belongs to the family of GalR-LacI repressors (6). Many proteins of this family areknown to autoregulate their own synthesis (8, 15, 28).This autoregulation is accomplished through the specific bindingof these proteins to the promoter region of their own genes (8,15). If, similar to these proteins, PtxS autoregulates its ownsynthesis in P. aeruginosa, the specific gel shift band that thePAO1 lysate produces with the 52-bp fragment may represent bindingof PtxS to its promoter region. To examine this possibility, wehave utilized P. aeruginosa PAO1::ptxS, which is a ptxS isogenicmutant of PAO1 (6). This mutant was constructed by the genereplacement technique as previously described (6). The constructionof the mutant was confirmed by Southern blot hybridization experimentsusing a specific ptxS probe (6; data not shown). Both PAO1and PAO1::ptxS were grown in TSB-DC medium, and the lysates wereexamined for 52-bp fragment binding activity. As seen in Fig.3A, the specific gel shift band was detected with the PAO1 lysateonly. Complementation experiments were conducted to confirm thatthe absence of the binding activity in the PAO1::ptxS lysate wasdue to the loss of ptxS. For these experiments, plasmid pAH56,which carries an intact copy of ptxS (9), was introduced intoPAO1::ptxS. A specific gel shift band was detected when the lysateof PAO1::ptxS/pAH56 was incubated with the 52-bp fragment (Fig.3A). This band parallels the typical gel shift band that we usuallydetect when the PAO1 lysate is incubated with the 52-bp fragment(Fig. 3A). These results suggest that ptxS contributes to theobserved binding to the ptxS upstream region.

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FIG. 3. Gel shift assays to determine if the DNA-protein complex that was detected with the 52-bp probe represents binding of PtxS to the ptxS upstream region. (A) The lysate from a ptxS isogenic mutant (PAO1::ptxS) resulted in no specific gel shift band. The gel shift band was regenerated when a plasmid (pAH56) carrying an intact copy of ptxS was introduced into the mutant. The 52-bp probe was incubated with either no lysate (lane 1), PAO1::ptxS lysate (lane 2), PAO1 lysate (lane 3), or PAO1::ptxS/pAH56 lysate (lane 4). Each reaction mixture contained 25 µg of cell lysate. (B) PtxS synthesized in E. coli (by the T7 expression system) binds specifically to the 52-bp probe. The lysate obtained from E. coli K38 containing either pJAC17 (ptxS expression plasmid) or pT7-5 (vector control) was incubated with the 52-bp probe. Lanes: 1, 52-bp probe alone; 2, 52-bp probe plus K38/pT7-5 lysate (10 µg); 3, 52-bp probe plus K38/pJAC17 lysate (3.0 µg); 4, 52-bp probe plus K38/pJAC17 lysate (1.5 µg); 5, 52-bp probe plus PAO1 lysate (25 µg). (C) Incubation of radiolabeled PtxS (using the T7 expression system) with the unlabeled 52-bp fragment. In parallel with the typical gel shift assay using the labeled 52-bp probe and K38/pJAC17 lysate (lanes 1 to 3), radiolabeled PtxS was incubated with the unlabeled 52-bp probe and assayed for binding activity (lane 5). The position of the band exactly parallels that of the typical gel shift band. Lanes: 1, labeled 52-bp probe alone; 2, 52-bp probe plus K38/pT7-5 lysate (10 µg); 3, 52-bp probe plus K38/pJAC17 lysate (3 µg); 4, labeled PtxS alone; 5, labeled PtxS plus unlabeled 52-bp fragment.

Confirmation of PtxS binding to the ptxS upstream region. The above-described results showed that a functional ptxS gene is required to produce the 52-bp fragment-specific bindingactivity. However, PtxS may either bind directly to the 52-bpfragment or induce another P. aeruginosa protein to bind. Thus,to confirm that the observed gel shift band is due to PtxS, weconducted additional gel shift experiments using the lysate ofE. coli K38/pJAC17, in which ptxS is expressed from the T7 promoter(6). Plasmid pJAC17 was constructed by cloning of the HincII-HindIIIfragment which carries the intact ptxS open reading frame in theSmaI-HindIII sites of pT7-5 (6). Expression experiments showedthat K38/pJAC17 produced a 38-kDa protein (6). Thus, PtxS wassynthesized in K38/pJAC17 using the previously described protocol(6) except that labeled cysteine and methionine were replacedwith unlabeled cysteine and methionine. K38 carrying the cloningvector pT7-5 was used as a negative control. As shown in Fig.3B, the lysate of K38/pT7-5 produced no gel shift band with the52-bp fragment, whereas the lysate of K38/pJAC17 produced thetypical gel shift band (Fig. 3B). To provide further evidencethat the binding protein in the lysate of K38/pJAC17 is PtxS,PtxS was selectively labeled by using ³⁵S-labeled cysteine and methionine as previously described. Thelysates of the labeled cells were incubated with the unlabeled52-bp fragment. In a parallel experiment, the lysate of K38/pJAC17that was prepared with unlabeled amino acids was incubated withthe ³²P-labeled 52-bp fragment. The incubation of the ³⁵S-labeled lysate with the unlabeled 52-bp fragment produced aspecific gel shift band (Fig. 3C). This band migrated in exactlythe same position as the typical gel shift band that was producedby incubation of the unlabeled lysate with the ³²P-labeled 52-bp fragment (Fig. 3C). These results strongly suggestthat the PtxS protein specifically binds to the ptxS upstreamregion.

Autoregulation of PtxS synthesis. After proving that PtxS binds specifically to the ptxS upstream region, it was important to determine if the binding of PtxScauses autoregulation of PtxS synthesis. To examine this possibility,we utilized the ptxS-lacZ fusion plasmid pBS8-4 (see Materialsand Methods for construction). Plasmid pBS8-4 was introduced intoboth PAO1 and PAO1::ptxS. PAO1/pBS8-4 and PAO1::ptxS/pBS8-4 weregrown in TSB-DC medium for 14 h, and the level of $beta$ -galactosidaseactivity was determined as previously described (16). As depictedin Fig. 4, the level of $beta$ -galactosidase activity produced by PAO1::ptxS/pBS8-4was four- to fivefold higher than that produced by PAO1/pBS8-4.These results suggest that PtxS negatively autoregulates its ownsynthesis in P. aeruginosa.

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FIG. 4. Autoregulation of ptxS expression in P. aeruginosa. Plasmid pBS8-4 (which carries a ptxS-lacZ fusion) was introduced into PAO1 and PAO1::ptxS. Cells were grown in TSB-DC medium for 14 h, and the level of $beta$ -galactosidase activity was determined as previously described (16). PAO1 carrying pSW205 (negative control) produced no $beta$ -galactosidase activity. The values are averages of three independent experiments ± the standard error of the mean.

Identification of the specific ptxS sequence to which PtxS binds. The precise ptxS sequence to which PtxS binds was identified by DNase I protection analysis as previously described usingPtxS synthesized by E. coli K38/pJAC17 (6). PtxS protecteda 20-bp region from DNase I digestion (Fig. 5A). Within the 20-bpprotected region, there is a 14-bp sequence of dyad symmetry (Fig.5B). We have confirmed that ptxS is expressed in E. coli by usinga ptxS-lacZ fusion (data not shown). However, we have not beenable to determine the ptxS transcriptional start site. Since ptxSis expressed in E. coli, we tried to determine if the ptxS promoterresembles the E. coli $sigma$ ⁷⁰ promoters (10). We have identified potential $-$ 10 and $-$ 35 sequenceswithin the 20-bp protected region. The $-$ 10 sequence (which islocated 97 bp from the GTG translation start codon) contains fourof the six bases (TATAAT) that are found within the $-$ 10 sequenceof $sigma$ ⁷⁰ promoters, whereas the $-$ 35 site contains five of the six bases(TTGACA) that are found within the $-$ 35 sequence of $sigma$ ⁷⁰ promoters (Fig. 5B). In addition, similar to that of $sigma$ ⁷⁰ promoters, the distance between the $-$ 10 and $-$ 35 sites is 17 bp(Fig. 5B).

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FIG. 5. Determination of the specific nucleotide sequence within the ptxS upstream region to which PtxS binds. (A) DNase I protection analysis of PtxS binding to the ptxS upstream region. The 103-bp fragment of the ptxS upstream region was singly end labeled with [ $gamma$ -³²P]ATP and incubated with increasing concentrations of E. coli K38/pJAC17 lysate in which ptxS was overexpressed from the T7 promoter. Lanes: 1, 103-bp probe; 2 to 4, 103-bp probe plus 10, 15, and 25 µg of lysate, respectively. All reaction mixtures were treated with DNase I. The complementary nucleotide sequence of the fragment is shown. In addition, specific nucleotides that constitute the DNase I-protected region are indicated on the right. (B) Nucleotide sequence of the ptxS upstream region. The solid line indicates the 20-bp DNase I-protected region. The 14-bp palindrome is shown by opposing arrows. The potential $-$ 10 and $-$ 35 sites (based on comparisons with $sigma$ ⁷⁰ promoters) are identified by dotted lines.

	DISCUSSION

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Results obtained in this study confirm that PtxS negatively autoregulates its synthesis in P. aeruginosa. Based on our previousanalysis, we have suggested that PtxS belongs to the GalR-LacIfamily of transcriptional repressors (6). The most significanthomology between PtxS and proteins of the GalR-LacI family iswithin the helix-turn-helix motif (DNA binding motif) (6).Among the different proteins within this family, three are knownto negatively autoregulate their own synthesis: the galactoseisorepressor GalS (28), the cytidine repressor CytR (8),and the purine regulon repressor PurR (15). Several previoustranscriptional studies have shown that the negative autoregulationof GalS, CytR, and PurR is weak (about two- to threefold) (8,15, 28). However, these studies utilized transcriptional fusionsthat were carried either in the chromosome or on low-copy-numberplasmids. For example, the level of galS expression from a galS-lacZfusion carried in the chromosome of an E. coli galS mutant wasincreased by twofold (28). Similarly, in a cytR mutant, thelevels of cytR expression from a cytR-lacZ fusion carried on alow-copy-number plasmid was increased by twofold (8). In comparison,the increase in the level of ptxS expression in PAO1::ptxS isslightly higher (four- to fivefold) (Fig. 4). The copy numberof the ptxS-lacZ fusion plasmid (pBS8-4), and other plasmids thatcarry the 1.8-kb PstI stability fragment (18, 30), is notknown. However, if the copy number of pBS8-4 is assumed to behigh, the autoregulation of PtxS is similar to that of CytR andGalS. Alternatively, if the copy number is low, the levels ofptxS autoregulation may be even more significant. Currently, weare constructing a ptxS-lacZ fusion by using the low-copy-number,broad-host-range lacZ transcriptional fusion vector pMP190 (21).This fusion should help us directly compare the levels of autoregulationbetween ptxS and the other three galR-lacIgenes.

The ptxS upstream region shares several characteristic features with the upstream regions of galS, cytR, and purR. For example,all three genes autoregulate their own synthesis by binding tospecific regions (operator sites) within their genes (8, 15,28). Many proteins of the GalR-LacI family bind to multipleoperator sites either within the upstream region or within thestructural region of the genes that they regulate (27). Thepresence of multiple operator sites is thought to be importantin augmenting the repression of the regulated genes (5). Forexample, galE, galS, galP, and galR are known to contain two operatorsites, i.e., one within the promoter region and another withinthe structural gene (29). The purR gene contains two operatorsites that are located downstream of the transcription initiationsite (15, 20). The cytR gene contains only one operator siteupstream of the transcription start site (8). Each operatorsite contains a consensus binding sequence that is specific foreach protein (8, 15, 20, 28). The nucleotides withinthese consensus sequences are arranged in dyad symmetry, or apalindrome, to allow their respective proteins to bind as dimers(29). As we have shown in this study, PtxS binds to a singlesite within the 103-bp fragment upstream of the GTG translationalstart codon (Fig. 5B). This ptxS binding region contains a 14-bppalindromic sequence that may represent a potential PtxS operatorsite (Fig. 5B). The 5' half of this palindromic sequence containsall three conserved nucleotides ( ... AAC) that are usually detectedwithin the DNA binding half sites for several proteins of theGalR-LacI family (27). The location of the PtxS operator sitewith respect to the ptxS transcriptional start site is not known.Despite several attempts, we were not able to determine the ptxStranscription start site. However, if ptxS has a $sigma$ ⁷⁰ promoter that utilizes the potential $-$ 10 and $-$ 35 sites that wehave identified (Fig. 5B), the ptxS transcriptional start sitemay be within the DNase I-protected region. If this proves tobe true, then unlike galS, purR, and cytR, the ptxS operator sitewould be within the ptxS transcriptional startsite.

PtxS may autoregulate its own synthesis by a mechanism that resembles those utilized by some proteins of the GalR-LacI family.However, the specific environmental signal to which PtxS responds,as well as the exact mechanism through which PtxS regulates itstarget genes (other than ptxS), is not known. Most proteins ofthe GalR-LacI family function in response to certain environmentalsignals called effectors. These effectors include carbohydrates,nucleosides, and modified amino acids (4, 27). Within thestructure of many of the GalR-LacI proteins, there are conservedregions to which different effectors may bind (27). As we haveshown previously, the strongest homology between PtxS and thedifferent GalR-LacI proteins is within the amino-terminal DNAbinding motif (6). Although a second region of homology hasbeen identified, this region does not involve the effector bindingsequences (6). The lack of conserved effector sequences withinPtxS suggests that the protein does not utilize the effector bindingsystem for its function. PtxS was originally identified throughits negative effect on exotoxin A synthesis (6). Exotoxin Asynthesis in P. aeruginosa is regulated by different environmentalsignals (especially iron, which negatively regulates toxA expression)(2, 13, 33). However, PtxS binding to its promoter wasnot affected by the presence of iron in the growth medium (datanot shown). Whether iron affects PtxS binding to other genes remainsto bedetermined.

With respect to the PtxS target gene, we have previously shown that ptxS modifies the function of the toxA transcriptionalactivator ptxR (6). The ptxS gene is divergently transcribedfrom ptxR from the opposite strand (6). Based on recent transcriptionalanalysis of ptxR (using a ptxR-lacZ fusion plasmid), we have suggestedthat PtxS may interfere with ptxR expression in P. aeruginosa(6). However, this effect is not likely to be accomplishedthrough direct binding of PtxS to the ptxR promoter. PtxS (thatwas produced in E. coli by the T7 expression system) did not bindto different segments of the ptxR upstream region (data not shown).In addition, computer analysis revealed that the ptxR upstreamregion lacks the 14-bp palindromic sequence (PtxS operator site)(data not shown). Therefore, it is possible that PtxS regulatesptxR expression through another regulatorygene.

	ACKNOWLEDGMENTS

This study was supported by a Public Health Service grant (AI-33386) to Abdul Hamood. Britta Swanson was supported by a researchfellowship from the Cystic FibrosisFoundation.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Immunology, Texas Tech University Health Sciences Center,Lubbock, TX 79430. Phone: (806) 743-1707. Fax: (806) 743-2334.E-mail: micanh{at}ttuhsc.edu.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Ausubel, F., R. Brent, R. Kingston, D. Moor, J. Seidman, J. Smith, and K. Strauhle. 1988. Current protocols in molecular biology. Wiley Interscience, New York, N.Y.

2. Bjorn, M. J., B. H. Iglewski, S. K. Ives, J. C. Sadoff, and M. L. Vasil. 1977. Effect of iron on yields of exotoxin A in cultures of Pseudomonas aeruginosa PA103. Infect. Immun. 19:785-791.

3. Bodey, G., R. Bolivar, V. Fainstein, and L. Jadeja. 1983. Infections caused by Pseudomonas aeruginosa. Rev. Infect. Dis. 5:297-313.

4. Bouchez, D., and J. Tourneur. 1991. Organization of the agropine synthesis region of the T-DNA of the Ri plasmid from Agrobacterium rhizogenes. Plasmid 25:27-39[Medline].

5. Choy, H. E., and S. Adhya. 1993. RNA polymerase idling and clearance in gal promoters: use of supercoiled mini-circle DNA template made in vivo. Proc. Natl. Acad. Sci. USA 90:472-476[Abstract/Free Full Text].

6. Colmer, J. A., and A. N. Hamood. 1998. Characterization of ptxS, a Pseudomonas aeruginosa gene which interferes with the effect of the exotoxin A positive regulatory gene, ptxR. Mol. Gen. Genet. 258:250-259[Medline].

7. Gambello, M. J., S. Kaye, and B. H. Iglewski. 1993. lasR of Pseudomonas aeruginosa is a transcriptional activator of the alkaline protease gene (apr) and enhancer of exotoxin A synthesis. Infect. Immun. 61:1180-1184[Abstract/Free Full Text].

8. Gerlach, P., P. Valentin-Hansen, and E. Bremer. 1990. Transcriptional regulation of the cytR gene of Escherichia coli: autoregulation and positive control by the cAMP/CAP complex. Mol. Microbiol. 4:479-488[Medline].

9. Hamood, A. N., J. A. Colmer, U. A. Ochsner, and M. L. Vasil. 1996. Isolation and characterization of a Pseudomonas aeruginosa gene, ptxR, which positively regulates exotoxin A production. Mol. Microbiol. 21:97-110[Medline].

10. Hawley, D. K., and W. R. McClure. 1983. Compilation and analysis of Escherichia coli promoter DNA sequences. Nucleic Acids Res. 11:2237-2255[Abstract/Free Full Text].

11. Holloway, B. W., V. Krishnapillai, and A. F. Morgan. 1979. Chromosomal genetics of Pseudomonas. Microbiol. Rev. 43:73-102[Free Full Text].

12. Iglewski, B. H., and D. Kabat. 1975. NAD-dependent inhibition of protein synthesis by Pseudomonas aeruginosa toxin. Proc. Natl. Acad. Sci. USA 2:2284-2288.

13. Liu, P. V. 1973. Exotoxin A of Pseudomonas aeruginosa. I. Factors that influence the production of exotoxin A. J. Infect. Dis. 128:506-513[Medline].

14. Lowry, O. H., N. J. Rosebrough, A. L. Farr, and R. J. Randall. 1951. Protein measurement with the Folin phenol reagent. J. Biol. Chem. 193:265-275[Free Full Text].

15. Meng, L. M., M. Kilstrup, and P. Nygaard. 1990. Autoregulation of PurR repressor synthesis and involvement of purR in the regulation of purB, purC, purL, purMN, and guaBA expression in Escherichia coli. Eur. J. Biochem. 187:373-379[Medline].

16. Miller, J. H. 1973. Experiments in molecular genetics Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

17. Ohman, D. E., J. C. Sadoff, and B. H. Iglewski. 1980. Exotoxin A-deficient mutants of Pseudomonas aeruginosa PA103: isolation and characterization. Infect. Immun. 28:899-908[Abstract/Free Full Text].

18. Olsen, R. H., G. DeBusscher, and W. R. McCombie. 1982. Development of broad-host-range vectors and gene banks: self-cloning of the Pseudomonas aeruginosa PAO chromosome. J. Bacteriol. 150:60-69[Abstract/Free Full Text].

19. Prince, R. W., C. D. Cox, and M. L. Vasil. 1993. Coordinate regulation of siderophore and exotoxin A production: molecular cloning and sequencing of the Pseudomonas aeruginosa fur gene. J. Bacteriol. 175:2589-2598[Abstract/Free Full Text].

20. Rolfes, R. J., and H. Zalkin. 1990. Autoregulation of Escherichia coli purR requires two control sites downstream of the promoter. J. Bacteriol. 172:5758-5766[Abstract/Free Full Text].

21. Spaink, H. P., R. J. H. Okker, C. A. Wijffelman, E. Pees, and B. J. J. Lugtenberg. 1987. Promoters in the nodulation region of the Rhizobium leguminosarum Sym plasmid pRL1J1. Plant Mol. Biol. 9:27-39.

22. Steel, R. G., and J. H. Torrie. 1980. Principles and procedures of statistics. A biometrical approach, 2nd ed. McGraw-Hill, Inc., New York, N.Y.

23. Storey, D. G., D. W. Frank, M. A. Farinha, A. M. Kropinski, and B. H. Iglewski. 1990. Multiple promoters control the regulation of the Pseudomonas aeruginosa regA gene. Mol. Microbiol. 4:499-503[Medline].

24. Storey, D. G., T. Raivio, D. W. Frank, M. J. Wick, S. Kaye, and B. H. Iglewski. 1991. Effect of regB on expression from P1 and P2 promoters of the Pseudomonas aeruginosa regAB operon. J. Bacteriol. 173:6088-6094[Abstract/Free Full Text].

25. Swanson, B. L., and A. N. Hamood. Unpublished data.

26. Tabor, S., and C. Richardson. 1985. A bacteriophage T7 RNA polymerase/promoter system for controlled exclusive expression of specific genes. Proc. Natl. Acad. Sci. USA 82:1074-1078[Abstract/Free Full Text].

27. Weickert, M. J., and S. Adhya. 1992. A family of bacterial regulators homologous to Gal and Lac repressors. J. Biol. Chem. 267:15869-15874[Abstract/Free Full Text].

28. Weickert, M. J., and S. Adhya. 1993. Control of transcription of the Gal repressor and isorepressor gene in Escherichia coli. J. Bacteriol. 175:251-258[Abstract/Free Full Text].

29. Weickert, M. J., and S. Adhya. 1993. The galactose regulon of Escherichia coli. Mol. Microbiol. 10:245-251[Medline].

30. West, S. E. H., H. P. Schweizer, C. Dall, A. K. Sample, and L. J. Runyen-Janecky. 1994. Construction of improved Escherichia-Pseudomonas shuttle vectors derived from pUC18/19 and sequence of the region required for their replication in Pseudomonas aeruginosa. Gene 148:81-86[Medline].

31. West, S. E. H., A. K. Sample, and L. J. Runyen-Janecky. 1994. The vfr gene product, required for Pseudomonas aeruginosa exotoxin A and protease production, belongs to the cyclic AMP receptor protein family. J. Bacteriol. 176:7532-7542[Abstract/Free Full Text].

32. White, B. A. 1993. PCR protocols: current methods and applications. Humana Press, Totowa, N.J.

33. Wick, M. J., D. W. Frank, D. G. Storey, and B. H. Iglewski. 1990. Structure, function, and regulation of Pseudomonas aeruginosa exotoxin A. Annu. Rev. Microbiol. 44:335-363[Medline].

34. Woods, R. E. 1976. Pseudomonas: the compromised host. Hosp. Pract. 11:91-100[Medline].

35. Woods, R. E., and B. H. Iglewski. 1983. Toxins of Pseudomonas aeruginosa: new perspectives. Rev. Infect. Dis. 5:S715-S722.

This article has been cited by other articles:

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	ALL ASM JOURNALS

1.	Ausubel, F., R. Brent, R. Kingston, D. Moor, J. Seidman, J. Smith, and K. Strauhle. 1988. Current protocols in molecular biology. Wiley Interscience, New York, N.Y.
2.	Bjorn, M. J., B. H. Iglewski, S. K. Ives, J. C. Sadoff, and M. L. Vasil. 1977. Effect of iron on yields of exotoxin A in cultures of Pseudomonas aeruginosa PA103. Infect. Immun. 19:785-791.
3.	Bodey, G., R. Bolivar, V. Fainstein, and L. Jadeja. 1983. Infections caused by Pseudomonas aeruginosa. Rev. Infect. Dis. 5:297-313.
4.	Bouchez, D., and J. Tourneur. 1991. Organization of the agropine synthesis region of the T-DNA of the Ri plasmid from Agrobacterium rhizogenes. Plasmid 25:27-39[Medline].
5.	Choy, H. E., and S. Adhya. 1993. RNA polymerase idling and clearance in gal promoters: use of supercoiled mini-circle DNA template made in vivo. Proc. Natl. Acad. Sci. USA 90:472-476[Abstract/Free Full Text].
6.	Colmer, J. A., and A. N. Hamood. 1998. Characterization of ptxS, a Pseudomonas aeruginosa gene which interferes with the effect of the exotoxin A positive regulatory gene, ptxR. Mol. Gen. Genet. 258:250-259[Medline].
7.	Gambello, M. J., S. Kaye, and B. H. Iglewski. 1993. lasR of Pseudomonas aeruginosa is a transcriptional activator of the alkaline protease gene (apr) and enhancer of exotoxin A synthesis. Infect. Immun. 61:1180-1184[Abstract/Free Full Text].
8.	Gerlach, P., P. Valentin-Hansen, and E. Bremer. 1990. Transcriptional regulation of the cytR gene of Escherichia coli: autoregulation and positive control by the cAMP/CAP complex. Mol. Microbiol. 4:479-488[Medline].
9.	Hamood, A. N., J. A. Colmer, U. A. Ochsner, and M. L. Vasil. 1996. Isolation and characterization of a Pseudomonas aeruginosa gene, ptxR, which positively regulates exotoxin A production. Mol. Microbiol. 21:97-110[Medline].
10.	Hawley, D. K., and W. R. McClure. 1983. Compilation and analysis of Escherichia coli promoter DNA sequences. Nucleic Acids Res. 11:2237-2255[Abstract/Free Full Text].
11.	Holloway, B. W., V. Krishnapillai, and A. F. Morgan. 1979. Chromosomal genetics of Pseudomonas. Microbiol. Rev. 43:73-102[Free Full Text].
12.	Iglewski, B. H., and D. Kabat. 1975. NAD-dependent inhibition of protein synthesis by Pseudomonas aeruginosa toxin. Proc. Natl. Acad. Sci. USA 2:2284-2288.
13.	Liu, P. V. 1973. Exotoxin A of Pseudomonas aeruginosa. I. Factors that influence the production of exotoxin A. J. Infect. Dis. 128:506-513[Medline].
14.	Lowry, O. H., N. J. Rosebrough, A. L. Farr, and R. J. Randall. 1951. Protein measurement with the Folin phenol reagent. J. Biol. Chem. 193:265-275[Free Full Text].
15.	Meng, L. M., M. Kilstrup, and P. Nygaard. 1990. Autoregulation of PurR repressor synthesis and involvement of purR in the regulation of purB, purC, purL, purMN, and guaBA expression in Escherichia coli. Eur. J. Biochem. 187:373-379[Medline].
16.	Miller, J. H. 1973. Experiments in molecular genetics Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
17.	Ohman, D. E., J. C. Sadoff, and B. H. Iglewski. 1980. Exotoxin A-deficient mutants of Pseudomonas aeruginosa PA103: isolation and characterization. Infect. Immun. 28:899-908[Abstract/Free Full Text].
18.	Olsen, R. H., G. DeBusscher, and W. R. McCombie. 1982. Development of broad-host-range vectors and gene banks: self-cloning of the Pseudomonas aeruginosa PAO chromosome. J. Bacteriol. 150:60-69[Abstract/Free Full Text].
19.	Prince, R. W., C. D. Cox, and M. L. Vasil. 1993. Coordinate regulation of siderophore and exotoxin A production: molecular cloning and sequencing of the Pseudomonas aeruginosa fur gene. J. Bacteriol. 175:2589-2598[Abstract/Free Full Text].
20.	Rolfes, R. J., and H. Zalkin. 1990. Autoregulation of Escherichia coli purR requires two control sites downstream of the promoter. J. Bacteriol. 172:5758-5766[Abstract/Free Full Text].
21.	Spaink, H. P., R. J. H. Okker, C. A. Wijffelman, E. Pees, and B. J. J. Lugtenberg. 1987. Promoters in the nodulation region of the Rhizobium leguminosarum Sym plasmid pRL1J1. Plant Mol. Biol. 9:27-39.
22.	Steel, R. G., and J. H. Torrie. 1980. Principles and procedures of statistics. A biometrical approach, 2nd ed. McGraw-Hill, Inc., New York, N.Y.
23.	Storey, D. G., D. W. Frank, M. A. Farinha, A. M. Kropinski, and B. H. Iglewski. 1990. Multiple promoters control the regulation of the Pseudomonas aeruginosa regA gene. Mol. Microbiol. 4:499-503[Medline].
24.	Storey, D. G., T. Raivio, D. W. Frank, M. J. Wick, S. Kaye, and B. H. Iglewski. 1991. Effect of regB on expression from P1 and P2 promoters of the Pseudomonas aeruginosa regAB operon. J. Bacteriol. 173:6088-6094[Abstract/Free Full Text].
25.	Swanson, B. L., and A. N. Hamood. Unpublished data.
26.	Tabor, S., and C. Richardson. 1985. A bacteriophage T7 RNA polymerase/promoter system for controlled exclusive expression of specific genes. Proc. Natl. Acad. Sci. USA 82:1074-1078[Abstract/Free Full Text].
27.	Weickert, M. J., and S. Adhya. 1992. A family of bacterial regulators homologous to Gal and Lac repressors. J. Biol. Chem. 267:15869-15874[Abstract/Free Full Text].
28.	Weickert, M. J., and S. Adhya. 1993. Control of transcription of the Gal repressor and isorepressor gene in Escherichia coli. J. Bacteriol. 175:251-258[Abstract/Free Full Text].
29.	Weickert, M. J., and S. Adhya. 1993. The galactose regulon of Escherichia coli. Mol. Microbiol. 10:245-251[Medline].
30.	West, S. E. H., H. P. Schweizer, C. Dall, A. K. Sample, and L. J. Runyen-Janecky. 1994. Construction of improved Escherichia-Pseudomonas shuttle vectors derived from pUC18/19 and sequence of the region required for their replication in Pseudomonas aeruginosa. Gene 148:81-86[Medline].
31.	West, S. E. H., A. K. Sample, and L. J. Runyen-Janecky. 1994. The vfr gene product, required for Pseudomonas aeruginosa exotoxin A and protease production, belongs to the cyclic AMP receptor protein family. J. Bacteriol. 176:7532-7542[Abstract/Free Full Text].
32.	White, B. A. 1993. PCR protocols: current methods and applications. Humana Press, Totowa, N.J.
33.	Wick, M. J., D. W. Frank, D. G. Storey, and B. H. Iglewski. 1990. Structure, function, and regulation of Pseudomonas aeruginosa exotoxin A. Annu. Rev. Microbiol. 44:335-363[Medline].
34.	Woods, R. E. 1976. Pseudomonas: the compromised host. Hosp. Pract. 11:91-100[Medline].
35.	Woods, R. E., and B. H. Iglewski. 1983. Toxins of Pseudomonas aeruginosa: new perspectives. Rev. Infect. Dis. 5:S715-S722.