Distinct Sensory Pathways in Vibrio cholerae El Tor and Classical Biotypes Modulate Cyclic Dimeric GMP Levels To Control Biofilm Formation

Quorum sensing (QS), or cell-cell communication in bacteria,is achieved through the production and subsequent response tothe accumulation of extracellular signal molecules called autoinducers(AIs). To identify AI-regulated target genes in Vibrio choleraeEl Tor (V. cholerae_El), the strain responsible for the currentcholera pandemic, luciferase expression was assayed in an AI^–strain carrying a random lux transcriptional reporter libraryin the presence and absence of exogenously added AIs. Twenty-threegenes were identified and shown to require the QS transcriptionfactor, HapR, for their regulation. Several of the QS-dependenttarget genes, annotated as encoding hypothetical proteins, infact encode HD-GYP proteins, phosphodiesterases that degradethe intracellular second messenger cyclic dimeric GMP (c-di-GMP),which is important for controlling biofilm formation. Indeed,overexpression of a representative QS-activated HD-GYP proteinin V. cholerae_El reduced the intracellular concentration ofc-di-GMP, which in turn decreased exopolysaccharide productionand biofilm formation. The V. cholerae classical biotype (V.cholerae_Cl), which caused previous cholera pandemics and isHapR^–, controls c-di-GMP levels and biofilm formationby the VieA signaling pathway. We show that the VieA pathwayis dispensable for biofilm formation in V. cholerae_El but thatrestoring HapR in V. cholerae_Cl reestablishes QS-dependent repressionof exopolysaccharide production. Thus, different pandemic strainsof V. cholerae modulate c-di-GMP levels and control biofilmformation in response to distinct sensory pathways.

INTRODUCTION

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INTRODUCTION

Over the past century, pandemic outbreaks of the diarrheal diseasecholera have been caused by only two Vibrio cholerae biotypes(11). The classical biotype (V. cholerae_Cl) was responsiblefor the sixth pandemic, which lasted from 1899 to 1923. Theetiological agent of the current seventh pandemic that beganin 1961 is V. cholerae El Tor (V. cholerae_El). V. cholerae isan aquatic organism and its life cycle includes only transientcolonization of the human small intestine. In humans, virulencefactors elicit diarrhea, which is often fatal to the host butis also critical for efficiently transmitting the bacteriumback into the environment (12). In marine habitats, V. choleraeis often found attached to other organisms in microbial communitiescalled biofilms (19, 20). Ingestion of contaminated water orfood is the mode of transmission into the human gastrointestinaltract. Understanding the mechanisms used by these two V. choleraebiotypes to control virulence factor production and biofilmformation, as well as understanding the factors responsiblefor the emergence of V. cholerae_El as the dominant biotype,have been the focus of active research for decades.

A bacterial cell-cell communication process called quorum sensing(QS) is used to control virulence and biofilm formation in V.cholerae_El (14, 34, 56). QS is accomplished through the synthesis,release, and subsequent detection of signaling molecules calledautoinducers (AIs). Extracellular AI levels increase proportionatelyto increasing cell density, so the detection of AIs allows bacteriato monitor their population numbers.

V. cholerae_El strain C6706 uses two AIs, called CAI-1 and AI-2,for QS (5, 16, 17, 34, 38, 39). At low cell density, in theabsence of CAI-1 and AI-2, the cognate sensor kinase receptors(CqsS and LuxP/Q, respectively) autophosphorylate and transferphosphate to the phosphotransfer protein LuxU (Fig. 1A). LuxUtransfers the phosphate to the response regulator LuxO. PhosphorylatedLuxO (LuxO $~$ P) in conjunction with ${sigma}$ ⁵⁴ activates the transcriptionof genes encoding four small RNAs (sRNAs) called Qrr1-4, forquorum-regulatory RNAs. The Qrr sRNAs, along with the sRNA chaperoneHfq, destabilize the mRNA encoding the transcription factorHapR (21, 31). Thus, under low-cell-density conditions, HapRprotein is not produced, so the expression of HapR-repressedgenes is permitted, while HapR-activated genes are not expressed.At high cell density, CqsS and LuxP/Q bind their cognate AIs,and this event switches the sensors from acting as kinases toacting as phosphatases. Phosphate is removed from LuxO via LuxU.Dephosphorylated LuxO no longer activates transcription of theqrr genes, and in the absence of the Qrr sRNAs, hapR mRNA istranslated into HapR protein. Thus, under high-cell-densityconditions, HapR binds target promoter DNAs and regulates geneexpression (14, 28, 34, 51, 55). In contrast to V. cholerae_Elstrains, which are predominantly HapR⁺, V. cholerae_Cl strainO395 carries a frameshift mutation in hapR preventing QS regulationof HapR-controlled genes (22).

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FIG. 1. Multiple regulatory pathways control biofilm formation in V. cholerae. (A) In V. cholerae_El, sensory inputs from two QS AIs, CAI-1 (squares) and AI-2 (circles), regulate HapR, which in turn modulates the levels of c-di-GMP, vps transcription, biofilm formation, and virulence. (B) In V. cholerae_Cl, the VieSAB sensory system, in response to an unknown signal (triangles), controls c-di-GMP levels to control vps transcription, biofilm formation, and virulence in a HapR-independent manner.

In V. cholerae_El, at high cell density, HapR represses the expressionof vpsT, which encodes VpsT, a transcriptional activator ofthe biosynthesis operons vpsA-K and vpsL-Q, leading to a reductionin biofilm formation (4, 14, 30, 52, 53). At high cell density,QS also controls the transcription of multiple genes encodingproteins involved in modulating the levels of the intracellularsecond messenger molecule bis-(3'-5')-cyclic dimeric GMP (c-di-GMP)(51). These are diguanylate cyclases that produce and phosphodiesterasesthat degrade c-di-GMP, respectively (for a review of c-di-GMP,see reference 41). Diguanylate cyclases have a conserved domainthat includes but is not limited to the sequence motif GGDEF.Phosphodiesterases contain either an EAL domain or an HD-GYPdomain. V. cholerae is predicted to encode 41 GGDEF proteins,22 EAL proteins, and 9 HD-GYP proteins (13). The cumulativeeffect of HapR control of this class of genes in V. cholerae_Elis to promote high levels of c-di-GMP at low cell density, contributingto biofilm formation, and low levels of c-di-GMP at high celldensity, causing a reduction in biofilms (Fig. 1A). By contrast,V. cholerae_Cl strain O395, which is naturally HapR^–, usesthe phosphodiesterase VieA, a component of the VieSAB system,to control c-di-GMP (Fig. 1B) (32, 48, 50). Recently, however,we showed that this V. cholerae_Cl strain responds to CAI-1 andAI-2 to control the levels of a GGDEF protein through a HapR-independentpathway (15).

The above observations suggest that V. cholerae_El and V. cholerae_Clcould use distinct sensory pathways to control c-di-GMP levelsand biofilm formation. To investigate this idea, in the currentstudy we identified four putative HD-GYP proteins that are activatedat high cell density by QS in V. cholerae_El. Consistent withthis assignment of their function, overexpression of one ofthese, the VCA0681 protein, reduced vps expression and, in turn,biofilm formation. Degradation of c-di-GMP by VCA0681 requiredthe canonical HD-GYP motif because mutation of this sequencehindered its capacity to destroy c-di-GMP and prevented therepression of vps transcription and biofilm formation. V. cholerae_Clencodes all of the HD-GYPs present in V. cholerae_El, and theintroduction of a functional HapR in V. cholerae_Cl restoredthe QS-dependent modulation of c-di-GMP levels and exopolysaccharideproduction. Conversely, the elimination of VieA in V. cholerae_Eldid not alter c-di-GMP signaling. Therefore, we propose thatthe different V. cholerae biotypes utilize distinct signal transductionpathways, QS in V. cholerae_El and VieA in V. cholerae_Cl, tocoordinate c-di-GMP production and biofilm formation.

MATERIALS AND METHODS

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MATERIALS AND METHODS

Bacterial strains and culture conditions. All V. cholerae strains used were derivatives of either wild-type(WT) V. cholerae_El C6706str (49) or WT V. cholerae_Cl O395str(10). These included V. cholerae_El ${Delta}$ luxO_El (SLS349), luxO D47E_El(SLS340), ${Delta}$ hapR_El (BH1543), ${Delta}$ hapR ${Delta}$ vieA_El (BH2728), ${Delta}$ vieA_El (JC1185),and ${Delta}$ cqsA ${Delta}$ luxS (BH1575) mutants as well as V. cholerae_Cl ${Delta}$ vieA_Cl(JC1176), HapR⁺ ${Delta}$ vieA_Cl (BH2744), and HapR⁺ WT V. cholerae_Cl(WT_Cl) (BH2683) mutants. Escherichia coli S17-1 ${lambda}$ pir (6) and ElectroMAXDH10B (Invitrogen) cells were used for cloning. Bacteria weregrown at 37°C with shaking, except for in bioluminescenceassays, which were performed on cultures grown at 30°C,and in biofilm assays, during which cultures were not shaken.The following antibiotics, purchased from Sigma, were used (concentrationsare given in parentheses in µg/ml): chloramphenicol (10),kanamycin (100), ampicillin (100) streptomycin (5000), and tetracycline(10). Expression of VCA0681, VCA0681FLAG, and VCA0681FLAG(D229A)was induced with 0.5 mM isopropyl-β-D-thiogalactopyranoside(IPTG; Sigma).

DNA manipulations. Standard protocols were used for all DNA manipulations (45).Restriction enzymes and T4 DNA ligase for cloning were purchasedfrom New England Biolabs (NEB), and Herculase enhanced DNA polymerasefor PCR amplification was purchased from Stratagene. Standardprotocols (46) were used to make deletion constructs, as wellas the HapR⁺ V. cholerae_Cl strains, which contained a copy ofthe V. cholerae_El hapR gene under the control of its own promoterat the lacZ site. Luciferase-based reporter plasmids were madeby amplifying the promoters of the genes encoding the VC1295,VC1348, VC2340, VCA0210, and VCA0931 proteins from WT V. cholerae_Eland cloning them into the pBBRlux vector (described previouslyin reference 31) by insertion into the SpeI and BamHI restrictionsites. The pVCA0681 and pVCA0681FLAG vectors were constructedby cloning vca0681, containing or lacking a C-terminal FLAGepitope tag, into the EcoRI and BamHI sites of pEVS143 (9).The pVCA0681FLAG(D289A) derivative was constructed using theQuikChange II XL site-directed mutagenesis kit (Stratagene)according the instructions of the manufacturer. Western blottingof total protein was performed with monoclonal anti-Flag M2-peroxidase(horseradish peroxidase) antibody (Sigma) as described by themanufacturer. The primer sequences used for plasmid constructionare available upon request.

Construction of the random lux transcriptional reporter library. The random lux transcriptional reporter library was constructedas follows. Briefly, genomic DNA from WT V. cholerae_El was partiallydigested with Sau3A1 (New England Biolabs), and fragments inthe size range from 1 to 2 kb were isolated by agarose gel purificationusing a QiaEx II gel extraction kit (Qiagen) and subsequentlyligated into the BamHI site of the promoterless lux transcriptionalplasmid described previously (31). The ligation mixture wastransformed into E. coli strain S17-1 ${lambda}$ pir, and the E. coli transformantswere conjugated with an AI-deficient V. cholerae_El ${Delta}$ cqsA ${Delta}$ luxSstrain (BH1575) to transfer the library.

Differential bioluminescence induction. A total of $~$ 40,000 V. cholerae_El ${Delta}$ cqsA ${Delta}$ luxS exconjugants werearrayed in microtiter plates in LB medium with a Genetix QPix2XT colony picker and incubated overnight. Approximately 10%of the clones produced light at a level 50-fold above backgroundand were presumed to contain active promoters. These cloneswere rearrayed into new microtiter plates, incubated overnight,and then combined at a 1:1 ratio with an overnight culture ofan AI-deficient strain (CAI-1^–, AI-2^–) and, in parallelin a separate microtiter plate, with an AI-proficient strain(CAI-1⁺, AI-2⁺). Cultures were diluted 1/300 and incubated withagitation at 30°C for 8 h. This time point was chosen toensure that strains had reached high cell density. Bioluminescenceand optical density at 600 nm (OD₆₀₀) were measured for eachculture by use of an EnVision XCite multilabel plate reader(Perkin Elmer), and candidate AI-regulated cultures that showeddifferential bioluminescence between the AI-deficient and AI-proficientcultures of $≥$ 3-fold were selected. Candidate AI-regulated cloneswere identified as targets if the clone displayed a similarbioluminescence regulation pattern and scale in a Wallac 1409liquid scintillation counter (Perkin Elmer) as described previously(34). Finally, the lux reporter plasmid from each AI-regulatedtarget clone was isolated from the V. cholerae_El ${Delta}$ cqsA ${Delta}$ luxS strainand electroporated into E. coli ElectroMAX DH10B cells (Invitrogen)for conjugation into V. cholerae WT_El, ${Delta}$ luxO_El, luxO D47E_El,and ${Delta}$ hapR_El strains. Bioluminescence/OD₆₀₀ (LUX/OD) was alsomeasured for these overnight cultures.

Bioluminescence assays. In coculture experiments, donor strains were combined at a 1:1ratio with recipients, diluted 1/300, and incubated for 8 h.Monocultures were incubated overnight. Absorbance and bioluminescencewere quantified thereafter. Bioluminescence measurements weremade on a Wallac 1409 counter, except for those shown below(see Fig. 3), which were obtained using an EnVision XCite readerand multiplied by 100 to adjust for differences in reader sensitivity.LUX/OD is defined as counts min^–1 ml^–1/OD₆₀₀.

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FIG. 3. HD-GYP activity represses V. cholerae_El vpsL expression and biofilm formation. Expression of vpsL-lux in a V. cholerae_El low-cell-density mutant (luxO D47E) carrying a vector control (first pair of bars) or a vector carrying VCA0681 (second pair of bars), VCA0681-FLAG (third pair of bars), or VCA0681(D289A)-FLAG (fourth pair of bars) was measured in the presence (black bars) or absence (white bars) of IPTG. The mean LUX/OD and the standard deviation of triplicate cultures diluted 1/00 and subsequently grown for 8 h are shown. (B) Western blot of the strains shown in panel A visualized with anti-FLAG antibodies. (C) Biofilm formation of static cultures of the strains shown in panel A incubated for 48 h.

Quantification of intracellular c-di-GMP levels. Relative levels of c-di-GMP/OD₆₀₀ were determined for overnightcultures of V. cholerae WT_El, ${Delta}$ luxO_El, and luxO D47E_El strainscarrying the vector pEVS141, pVCA0681, or pVCA0681(D289A) aswell as for V. cholerae WT_Cl, HapR⁺ WT_Cl, ${Delta}$ vieA_Cl, and HapR⁺ ${Delta}$ vieA_Cl strains and the HapR⁺ ${Delta}$ vieA_Cl strain carrying pVCA0681.Tandem high-pressure liquid chromatography-mass spectrometrywas used to determine the relative levels of c-di-GMP, and theOD₆₀₀ was also determined as described previously (51).

Biofilm formation. Static 5-ml cultures of 1/100 dilutions of overnight cultureswere incubated in LB containing chloramphenicol and IPTG whereappropriate. The formation of a pellicle at the air-broth interfacewas assessed after $~$ 48 h.

RESULTS

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RESULTS

Identification of AI-regulated genes in V. cholerae_El. To identify QS-regulated genes in the V. cholerae_El strain C6706,we employed a strategy that simulated the gradual accumulationof AIs in cultures grown from low to high cell densities. Alibrary of random V. cholerae_El genomic fragments fused to apromoterless luciferase cassette (Materials and Methods) wastransformed into an AI-deficient V. cholerae_El strain. The transcriptionalfusion library was then screened for genes controlled by AIsby combining overnight cultures of the candidates at a 1:1 ratiowith an overnight culture of an AI-deficient V. cholerae_El strain(CA-1^–, AI-2^–) and, in parallel, with an AI-proficientV. cholerae_El strain (CAI-1⁺, AI-2⁺). Twenty-four unique candidategenes were identified that were differentially regulated $≥$ 3-fold(Table 1).

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TABLE 1. AI-controlled target genes in V. cholerae

To verify QS regulation, each candidate reporter plasmid wastransformed into WT V. cholerae_El and into various QS mutantsthat are "locked" either in the low-cell-density or in the high-cell-densitymode. The "locked" low-cell-density mutant luxO D47E_El carriesa constitutively active allele of luxO mimicking LuxO $~$ P and thereforeoverexpress the qrr genes, which repress hapR mRNA (Fig. 1A).By contrast, the ${Delta}$ luxO_El mutant mimics high cell density becausethe qrr genes are not expressed, and HapR is produced constitutively.As anticipated, AI-activated targets were highly expressed inthe WT and ${Delta}$ luxO strains, while AI-repressed targets were highlyexpressed in the luxO D47E and ${Delta}$ hapR strains (Table 1). Becauseeach candidate exhibited a similar expression pattern in a luxOD47E strain and a ${Delta}$ hapR strain that both simulate low cell density,our interpretation is that expression of each target gene isdependent on LuxO $~$ P as well as HapR. There was one exception.One QS target gene annotated VCA0939, encoding a GGDEF protein,was AI repressed and required LuxO $~$ P, but not HapR, for its control(15).

Because we and others are studying the link between QS and c-di-GMPin V. cholerae_El and V. cholerae_Cl (3, 15, 51), of particularinterest to us were two of the target genes identified in thisscreen, vca0681 and vca0895 (AI activated $~$ 8-fold and $~$ 7-fold,respectively) (Table 1). vca0895 was previously identified asAI activated in a microarray study (56), and both vca0895 andvca0681 are predicted to encode proteins that are annotatedas hypothetical. Our inspection of VCA0681 and VCA0895 showthey encode proteins containing HD-GYP domains, presumably withc-di-GMP phosphodiesterase activity. Only one HD-GYP protein,RpfG, from Xanthomonas has been studied to date (8, 43, 44).We scanned the V. cholerae_El genome for homologs of RpfG. Sevenproteins had high similarity; the two we identified (the VCA0681and VCA0895 proteins) and five additional proteins (the VC1295,VC1348, VC2340, VCA0210, and VCA0931 proteins). The VC2497 proteinalso showed reasonable similarity to RpfG but it lacked severalof the residues critical for phosphodiesterase activity andwas not considered further.

Alignment of the seven putative HD-GYP proteins to RpfG showsthat each contains the conserved HD and GYP residues as wellas several other residues identified in the consensus sequencethat are predicted to be important for phosphodiesterase activity(see Fig. S1 in the supplemental material) (13). The divergencein the N termini of the proteins is consistent with the modulardomain architecture of other proteins involved in controllingc-di-GMP levels, with potential N-terminal signaling domainsand C-terminal catalytic domains.

To determine whether any of the five genes not originally identifiedin our screen are controlled by QS, we constructed lux transcriptionalfusions to each and measured expression by the above-describedV. cholerae_El QS "locked" mutants. In addition to vca0681-luxand vca0895-lux, two other HD-GYP reporter fusions, vc2340-luxand vca0210-lux, are more highly expressed ( $~$ 32-fold and $~$ 9-fold,respectively) in WT_El and the locked high-cell-density mutant(the ${Delta}$ luxO_El mutant) than in the low-cell-density mutant (theluxO D47E_El mutant) (Fig. 2). Thus, expression of genes encodingfour of the seven HD-GYP proteins in V. cholerae_El is activatedby QS at high cell density. Consistent with this finding, wenote that vc2341, which is located adjacent to vc2340, and vca0211,which is located adjacent to vca0210, were previously identifiedas QS-activated genes (Table 1) (56). The remaining three fusionsto genes encoding HD-GYP proteins (VC1295, VC1348, and VCA0931)either were not expressed or were not regulated by QS underour conditions, and they were not pursued further. Neither vc2340nor vca0210 was identified in the genetic screen. We also didnot identify vpsL, a known AI-controlled target. Thus, we suspectthat the screen is not saturated in spite of several targetgenes having been identified multiple times (Table 1).

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FIG. 2. QS activates expression of four genes encoding HD-GYP proteins in V. cholerae. Expression of lux transcriptional fusions to the promoters of genes encoding predicted HD-GYP proteins was measured in the high-cell-density (WT and ${Delta}$ luxO) and low-cell-density (luxO D47E) strains. Shown in each panel are the mean LUX/OD and the standard deviation from triplicate overnight cultures.

HD-GYP activity represses V. cholerae vps expression and biofilm formation. QS control of multiple GGDEFs and EALs results in increasedc-di-GMP at low cell densities and decreased c-di-GMP at highcell densities (51). c-di-GMP levels correlate with expressionof the vps biosynthetic gene cluster. Thus, at high cell density,when c-di-GMP levels decline, vps transcription decreases (14,51). Our present results suggest that if QS increases the productionof four HD-GYP proteins at high cell density, because HD-GYPproteins degrade c-di-GMP, their activity could likewise contributeto the reduction in c-di-GMP and biofilm formation that occursat high cell density. To test this idea, we examined whetherthe phosphodiesterase activity of the HD-GYP proteins identifiedin the screen, VCA0681 and VCA0895, influenced vps expressionand biofilm formation. To do this, VCA0681 and VCA0895 wereoverexpressed in V. cholerae luxO D47E_El carrying either a vpsL-luxor a vpsT-lux transcriptional reporter. Overexpression of VCA0895inhibited growth, which prevented our determination of its effects.Overexpression of VCA0681 reduced expression of both vpsL-lux(Fig. 3A) and vpsT-lux (data not shown). Deletion of eithervca0681 or vca0895 from the V. cholerae_El genome did not altervps expression or biofilm formation. This latter result wasnot unexpected, due to the extreme redundancy of phosphodiesterases.

Phosphodiesterase activity of Xanthomonas campestris RpfG requiresthe conserved His (H231) and Asp (D232) residues (43). We mutatedthe corresponding Asp in the VCA0681 protein to an Ala (D289A)and examined its effects (see Fig. S1 in the supplemental material).To monitor protein expression, a FLAG epitope tag was introducedat the C terminus. The FLAG tag that was added to the WT VCA0681protein did not interfere with the repression of vpsL-lux (Fig.3A). However, mutation of the active site (D289A) eliminatedVCA0681 repression of vpsL-lux (Fig. 3A). Western blots showedthat both the WT and mutant proteins were produced at similarlevels (Fig. 3B). Thus, the putative active site of VCA0681is required for its repression of vpsL.

To determine whether VCA0681 protein-mediated repression ofvps transcription is sufficient to alter biofilm formation,we monitored biofilm pellicle formation in the V. cholerae luxOD47E_El strain carrying either VCA0681 or the active-site mutant.Consistent with the vps transcription results, biofilm formationwas repressed by the WT VCA0681 protein but not the mutant protein(Fig. 3C). These results show that the phosphodiesterase activityof the representative protein we examined, VCA0681, is sufficientto reduce biofilm formation. At high cell density, AI activationof expression of vca0681 and genes encoding three other HD-GYPproteins likely contributes to the role QS plays in controllingbiofilm formation (see Discussion).

The VCA0681 protein degrades c-di-GMP in V. cholerae_El. To determine whether the decreased vps expression and reducedbiofilm phenotype we observe as HD-GYP controlled (Fig. 3) areindeed a consequence of an HD-GYP-mediated reduction in c-di-GMPat high cell density, we measured c-di-GMP in V. cholerae_Elexpressing either VCA0681 or the active-site mutant (D289A).In high-cell-density overnight cultures, both the WT V. cholerae_Eland ${Delta}$ luxO_El strains had low c-di-GMP levels (Fig. 4). By contrast,the "locked" low-cell-density strain, luxO D47E_El, possessed $~$ 10-fold more c-di-GMP. When VCA0681 is overexpressed in thelow-cell-density luxO D47E_El mutant, c-di-GMP is reduced tolevels similar to those present in the WT V. cholerae_El and ${Delta}$ luxO_El high-cell-density strains. Expression of the active-sitemutant (D289A) in the luxO D47E strain has little effect onc-di-GMP levels, consistent with the impaired ability of thisactive-site mutant protein to repress vpsL expression or biofilmformation (Fig. 3).

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FIG. 4. The VCA0681 protein controls c-di-GMP levels in V. cholerae_El. Relative c-di-GMP/1,000·OD₆₀₀ (c-di-GMP concentration) in V. cholerae_El WT, ${Delta}$ luxO, and luxO D47E strains and in the luxO D47E strain carrying IPTG-inducible vectors harboring VCA0681 or VCA0681(D289A). Shown are the mean values for triplicate cultures, with error bars indicating the standard deviation of the mean.

V. cholerae_Cl modulates c-di-GMP levels by a mechanism different from that of V. cholerae_El. It has been proposed that the emergence of the V. cholerae_Elbiotype stems from its increased environmental fitness relativeto the classical biotype (23). V. cholerae_El strain C6076 witha mutation in the hapR gene, because it is locked in the low-cell-density,low-c-di-GMP mode, is enhanced for vps production and producesrobust biofilms (14, 56). By contrast, V. cholerae_Cl strainO395, which is naturally HapR^–, does not produce strongbiofilms. In this V. cholerae_Cl strain, deletion of the geneencoding the EAL protein VieA results in elevated vps expressionand biofilm formation (50) The phosphodiesterase VieA is a componentof the VieSAB signaling system that controls c-di-GMP levelsand hence vps expression and biofilm formation in V. cholerae_Cl(32, 48, 50). While VieA controls >100 genes in V. cholerae_Cl,the role of VieA in V. cholerae_El appears to be minor (1). Becausethe ability to produce enhanced exopolysaccharide is correlatedwith enhanced environmental survival, we explored the relativeimportance of the QS and VieA signaling systems in biofilm formationin these two biotypes.

We constructed all possible combinations of V. cholerae_El andV. cholerae_Cl HapR^+/– and VieA^+/– strains. As apreliminary test for the function of HapR in each strain, weexamined the canonical target luxCDABE, encoding luciferase,which is activated at high cell density in WT V. cholerae_Elbut not in an isogenic ${Delta}$ hapR mutant (34). luxCDABE is not expressedin the V. cholerae_Cl parent; however, density-dependent activationof luxCDABE is restored in the HapR⁺ V. cholerae_Cl strain (seeFig. S2 in the supplemental material). Thus, the presence ofHapR in V. cholerae_Cl restores HapR-dependent QS, at least withrespect to luciferase.

To test whether the reintroduction of HapR in V. cholerae_Clcould likewise restore the HapR-dependent repression of vpstranscription, we examined the expression of vpsL. As a reference,we measured vps transcription in the corresponding HapR⁺ andHapR^– V. cholerae_El strains. Deletion of the hapR genein V. cholerae_El enhanced vpsL expression 10-fold (Fig. 5A)(14). WT V. cholerae_Cl (HapR^–) exhibits modest basal levelexpression of vps, and transcription is repressed $~$ 100-fold inHapR⁺ V. cholerae_Cl (Fig. 5A). These results show that the lossof hapR in either V. cholerae_El or V. cholerae_Cl relieves QS-dependentrepression of vps transcription. Importantly, the absolute levelof vps expression in the HapR^– V. cholerae_El strain (Fig.5A) is nearly 100 times higher than that of WT (HapR^–)V. cholerae_Cl strain (Fig. 5A), consistent with the respectivebiofilm capabilities of the HapR^– V. cholerae_El mutantand the naturally HapR^– V. cholerae_Cl strain.

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FIG. 5. Expression of vpsL and levels of c-di-GMP are controlled differently in V. cholerae_El and V. cholerae_Cl. (A and B) Expression of vpsL-lux (A) and relative c-di-GMP levels (B) were measured for V. cholerae_El and V. cholerae_Cl strains containing or lacking hapR, and containing or lacking vieA. (C) Expression of vpsL-lux in V. cholerae_Cl ${Delta}$ vieA and ${Delta}$ vieA HapR⁺ strains carrying an IPTG-inducible vector expressing VCA0681 without or with IPTG. LUX/OD and c-di-GMP/1,000·OD₆₀₀ (c-di-GMP concentration) are shown for triplicate cultures, with error bars indicating the standard deviation of the mean.

We carried out an analogous set of experiments to assess therole of VieA in both V. cholerae_El and V. cholerae_Cl. Mutationof vieA in either HapR⁺ or HapR^– V. cholerae_El did notchange vpsL expression (Fig. 5A). By contrast, mutation of vieAin V. cholerae_Cl enhanced vps transcription in both the HapR⁺and HapR^– strains (Fig. 5A) (50). Thus, VieA appears capableof controlling c-di-GMP and biofilms only in V. cholerae_Cl,whereas HapR can function in both biotypes.

In both V. cholerae_El and V. cholerae_Cl, elevated levels ofvpsL and hence increased biofilms are a consequence of higherlevels of c-di-GMP. Consistent with this, we found that thevpsL expression patterns we observed in the eight V. cholerae_Eland V. cholerae_Cl strains (Fig. 5A) correlated with c-di-GMPlevels. That is, high-level vps expression tracked with increasedlevels of c-di-GMP (compare Fig. 5A to 5B). The one exceptionto this pattern is that the extreme repression of vpsL in HapR⁺V. cholerae_Cl is not mirrored by an equally drastic reductionin c-di-GMP. These results are consistent with our previousobservations for V. cholerae_El that HapR represses vpsL transcriptionnot only by a mechanism requiring c-di-GMP but also by repressingvpsT transcription directly through binding to the vpsT promoter(51). The HapR binding sites in the vpsT promoter region areidentical in both V. cholerae_El and V. cholerae_Cl, and thus,the HapR-dependent repression of vpsL transcription we observedfor V. cholerae_Cl may be due to this conserved c-di-GMP-independentregulatory mechanism. It remains possible, however, that thisresult occurred because we were at the lower limit of detectionof c-di-GMP in V. cholerae_Cl.

We wondered whether we could override VieA control of vps inV. cholerae_Cl by artificially manipulating c-di-GMP levels throughthe induction of HD-GYP production in the VieA^– V. cholerae_Clstrains. When VCA0681 expression was induced in a VieA^–V. cholerae_Cl strain, vps levels decreased to the levels ofthe VieA⁺ V. cholerae_Cl strain (Fig. 5C). In HapR⁺ V. cholerae_Cl,expressing VCA0681 from a vector had less effect on vps expressionthan endogenous expression of vieA (compare results in Fig.5C to those in Fig. 5A). Thus, VCA0681 cannot fully rescue aVieA defect in the HapR⁺ V. cholerae_Cl background. Nonetheless,the effect we did observe was mediated by c-di-GMP, becausec-di-GMP levels were also reduced to background levels whenVCA0681 is expressed (data not shown). We conclude that HD-GYPproteins, which are activated by HapR in V. cholerae_El strainC6706, may participate in both biotypes to control biofilm formationby altering c-di-GMP levels.

DISCUSSION

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DISCUSSION

Multiple HapR-dependent GGDEFs and EALs participate in regulatingthe levels of c-di-GMP, which links QS to the control of biofilmformation in V. cholerae_El strain C6706 (14, 51). In the presentwork, we discovered that four AI-activated (i.e., HapR-activated)genes annotated in the genome as hypothetical are in fact genesfor proteins with HD-GYP motifs predicted to encode phosphodiesterasesthat degrade c-di-GMP. The genes encoding these HD-GYPs arealso present in the V. cholerae_Cl O395 genome, yet this strainis naturally HapR^–. Thus, it was not obvious whether theHD-GYPs could impinge on c-di-GMP-mediated control of biofilmformation in V. cholerae_Cl. The difference in QS circuitry betweenthe two V. cholerae biotypes prompted us to characterize thecontribution of HapR, HD-GYP activity, c-di-GMP, and VieA tobiofilm formation in V. cholerae_El and V. cholerae_Cl. Specifically,we showed that (i) proteins with an HD-GYP domain can alterbiofilm formation in V. cholerae by reducing levels of c-di-GMP;(ii) an intact HD-GYP domain is required for this activity;(iii) HD-GYP proteins, although not activated by HapR in V.cholerae_Cl, when expressed are nonetheless capable of reducingc-di-GMP levels and exopolysaccharide production in this biotype;and (iv) HapR is capable of controlling c-di-GMP levels andbiofilm formation in both biotypes, whereas a major input fromVieA appears restricted to the V. cholerae_Cl biotype. Basedon the results presented here, we suggest that c-di-GMP modulatoryproteins play a role in biofilm formation in both V. cholerae_Eland V. cholerae_Cl but that the signaling pathways controllingtheir activities differ in the two biotypes. The predominantsensory system governing the c-di-GMP/biofilm pathway in V.cholerae_El is the HapR-dependent QS circuit, while in V. cholerae_Cl,the VieA system is the primary sensory input (Fig. 1).

How the sensory information from the network of multiple diguanylatecyclases and phosphodiesterases in V. cholerae and other bacteriais integrated to produce a specific response mediated by c-di-GMPis poorly understood. Current theories include mechanisms fortemporal control of diguanylate cyclase and phosphodiesterasegene expression, environmental control of the enzyme activities,discrete enzyme localization, and also feedback inhibition byc-di-GMP (42). V. cholerae_El was predicted by Galperin et al.(13) to encode 72 proteins that modulate c-di-GMP levels: 41diguanylate cyclases (GGDEFs) and 31 phosphodiesterases (22EALs and 9 HD-GYPs). Inactivation of a single diguanylate cyclaseor phosphodiesterase rarely results in a dramatic phenotypicchange, suggesting that phenotypes are observed only for strainsin which multiple genes encoding c-di-GMP regulatory enzymeshave been mutated. Alternatively, deletion of a single diguanylatecyclase or phosphodiesterase could produce a biofilm phenotypeonly under particular growth conditions or could alter a phenotypeunrelated to biofilm formation. A few notable exceptions includegenes encoding individual GGDEF proteins (CdgC, RocS, and MbaA)that, when mutated, produce an observable reduction in biofilmformation in V. cholerae_El grown under conditions similar tothose in this study (2, 40). Even though many GGDEFs, EALs,and HD-GYPs are present in V cholerae_Cl, VieA appears to bethe predominant EAL contributing to vps expression and biofilmformation, based on current studies (29, 50).

Our results suggest that the relative contributions of QS andVieA to the control of c-di-GMP vary between V. cholerae_El andV. cholerae_Cl (Fig. 1). In HapR⁺ V. cholerae_El, four HD-GYPsare expressed at high cell density. In conjunction with theGGDEFs and EALs described previously (51), the combined activitiesof these enzymes function to decrease c-di-GMP concentration,which reduces vps expression and terminates the formation ofbiofilms. HapR also represses toxin-coregulated pilin and choleratoxin production at high cell density in V. cholerae_El (34,56). Together, these results are consistent with a model inwhich high-cell-density conditions in the host intestine promotedecreased c-di-GMP levels, reduced biofilm formation, and thetermination of toxin-coregulated pilin and cholera toxin production(14, 55). The synchronous termination of these factors enhancesthe transmission of V. cholerae_El from the intestine back intothe environment. By contrast, c-di-GMP levels and biofilm formationare not repressed at high cell density in the naturally HapR^–V. cholerae_Cl biotype. A possible role for QS in transmissionpredicts that strains of V. cholerae that are HapR⁺ (e.g., V.cholerae_El strain C6706) and HapR^– (V. cholerae_Cl strainO395) should colonize with similar efficiencies at low celldensity. However, upon the attainment of high cell density inthe host intestine, QS in the HapR⁺ El Tor strains promotesdetachment and transmission into the environment, while thelack of HapR in strains like V. cholerae_Cl hinders detachmentand release from the host. Currently, however, there are noanimal models to measure transmission differences between V.cholerae biotypes.

Environmental and clinical isolates of both V. cholerae_El andV. cholerae_Cl often contain nonfunctional HapR proteins (14,22). We have previously proposed that such mutations could occurunder conditions in which the cost incurred from the loss ofHapR-mediated QS is outweighed by the gain provided by enhancedattachment via biofilm formation (14). This hypothesis wouldalso predict that strains of V. cholerae_Cl should be isolatedwith nonfunctional VieA proteins, because they would produceincreased exopolysaccharide and more-robust biofilms (Fig. 5A).However, we are aware of no incidences of natural VieA^–V. cholerae_Cl isolates. Thus, we suspect that altered expressionof some HapR-regulated target gene(s) in V. cholerae_El thatis not involved in production of exopolysaccharide providesa selective advantage for HapR^– V. cholerae. Based onthese observations, we predict that such a putative target gene(s)is HapR regulated but not VieA regulated. We are currently measuringthe selective advantage provided to QS⁺ compared to QS^–strains under different growth conditions to identify such atarget gene(s).

The history of cholera pandemics provides a model for studyingthe molecular mechanisms governing the emergence and reemergenceof bacterial pathogens. In spite of the fact that clinical symptomscaused by V. cholerae_El are less severe than those caused byV. cholerae_Cl, V. cholerae_El appears to have outcompeted V.cholerae_Cl during the current pandemic (26). It has been proposedthat this occurred because of the increased environmental fitnessof V. cholerae_El (23), the differential susceptibility to lyticphages between the biotypes (47), or the ability of V. cholerae_Elto more productively utilize carbohydrates such as chitin, whichV. cholerae metabolizes when associated with zooplankton inthe environment (33, 54). Many studies have examined the differencesbetween these two important pandemic biotypes in terms of virulencegenes and their expression (1, 7, 10, 18, 24, 25, 27, 36, 37),but less attention has been given to understanding the differencesin biofilm formation between different V. cholerae biotypes(1, 35). Because the life cycle of V. cholerae includes onlytransient colonization of the human host, a better understandingof the selective pressures driving the evolution of this pathogenin aquatic habitats where vibrios are autochthonous memberscould contribute to our understanding of pandemic strains. Environmentalattachment is proposed to be a crucial factor in the survivalof V. cholerae in natural systems; therefore, understandingthe signal transduction mechanisms controlling biofilm formationby V. cholerae in pathogenic and marine niches should shed lighton the mechanisms underlying the emergence and reemergence ofthis infectious pathogen.

ACKNOWLEDGMENTS

We thank J. Cong for strain construction and W. Ng for assistancewith c-di-GMP quantification.

This work was supported by HHMI, by NIH grants 5R01GM065859and 5R01A1054442, by NSF grant MCB-0343821 to B.L.B., and byan NIH postdoctoral fellowship (F32-AI054033-01) to B.K.H.

FOOTNOTES

* Corresponding author. Mailing address: Howard Hughes Medical Institute, Department of Molecular Biology, Princeton University, Princeton, NJ 08544-1014. Phone: (609) 258-2857. Fax: (609) 258-2957. E-mail: bbassler{at}princeton.edu

Published ahead of print on 24 October 2008.

Supplemental material for this article may be found at http://jb.asm.org/.

Present address: School of Biology, Georgia Institute of Technology,Atlanta, GA 30332-0230.

REFERENCES

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