Cell Density Modulates Acid Adaptation in Streptococcus mutans: Implications for Survival in Biofilms

doi:10.1128/JB.183.23.6875-6884.2001

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Journal of Bacteriology, December 2001, p. 6875-6884, Vol. 183, No. 23
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.23.6875-6884.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Cell Density Modulates Acid Adaptation in Streptococcus mutans: Implications for Survival in Biofilms

Yung-Hua Li,¹ Michael N. Hanna,¹ Gunnel Svensäter,² Richard P. Ellen,¹ and Dennis G. Cvitkovitch¹^,^*

Dental Research Institute, University of Toronto, Toronto, Ontario M5G 1G6, Canada,¹ and Department of Oral Microbiology, Malmö University, S-21421 Malmö, Sweden²

Received 26 June 2001/Accepted 7 September 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Streptococcus mutans normally colonizes dental biofilms and is regularly exposed to continual cycles of acidic pH during ingestionof fermentable dietary carbohydrates. The ability of S. mutansto survive at low pH is an important virulence factor in the pathogenesisof dental caries. Despite a few studies of the acid adaptationmechanism of this organism, little work has focused on the acidtolerance of S. mutans growing in high-cell-density biofilms.It is unknown whether biofilm growth mode or high cell densityaffects acid adaptation by S. mutans. This study was initiatedto examine the acid tolerance response (ATR) of S. mutans biofilmcells and to determine the effect of cell density on the inductionof acid adaptation. S. mutans BM71 cells were first grown in brothcultures to examine acid adaptation associated with growth phase,cell density, carbon starvation, and induction by culture filtrates.The cells were also grown in a chemostat-based biofilm fermentorfor biofilm formation. Adaptation of biofilm cells to low pH wasestablished in the chemostat by the acid generated from excessglucose metabolism, followed by a pH 3.5 acid shock for 3 h. Bothbiofilm and planktonic cells were removed to assay percentagesof survival. The results showed that S. mutans BM71 exhibiteda log-phase ATR induced by low pH and a stationary-phase acidresistance induced by carbon starvation. Cell density was foundto modulate acid adaptation in S. mutans log-phase cells, sincepre-adapted cells at a higher cell density or from a dense biofilmdisplayed significantly higher resistance to the killing pH thanthe cells at a lower cell density. The log-phase ATR could alsobe induced by a neutralized culture filtrate collected from alow-pH culture, suggesting that the culture filtrate containedan extracellular induction component(s) involved in acid adaptationin S. mutans. Heat or proteinase treatment abolished the inductionby the culture filtrate. The results also showed that mutantsdefective in the comC, -D, or -E genes, which encode a quorumsensing system essential for cell density-dependent inductionof genetic competence, had a diminished log-phase ATR. Additionof synthetic competence stimulating peptide (CSP) to the comCmutant restored the ATR. This study demonstrated that cell densityand biofilm growth mode modulated acid adaptation in S. mutans,suggesting that optimal development of acid adaptation in thisorganism involves both low pH induction and cell-cellcommunication.

	INTRODUCTION

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Streptococcus mutans is an oral bacterium that depends on a "biofilm life-style" for survival and persistence in its naturalecosystem, dental plaque (43). Under appropriate environmentalconditions, this bacterium can rapidly produce acid from fermentabledietary carbohydrates and initiate demineralization of the toothsurface (7). S. mutans is therefore considered an importantetiological agent of dental caries (34). The environmental conditionsencountered by S. mutans in dental biofilms are highly variable,including frequent shifts in pH from above 7.0 to as low as 3.0during the ingestion of dietary carbohydrates by the host (16).Thus, pH exerts a significant ecological pressure on S. mutans,and its ability to tolerate and grow in low-pH environments iscrucial to its survival andpathogenicity.

Considerable evidence indicates that S. mutans has evolved several mechanisms to survive the pH changes encountered in plaque.The best characterized include proton extrusion by proton-translocatingF(H⁺)-ATPase efflux (2, 24) and expulsion of acid end-products(10). Other mechanisms include decreased proton permeability(1), increased synthesis of chaperonins (29), increased expressionof the ffh gene involved in targeting of membrane-associated proteins(21), changes in membrane fatty acid composition (52), andup-regulation of DNA repair systems (22, 26).

Studies using continuous cultures first showed that during a shift to acidic pH, survival of S. mutans was enhanced when theexternal pH was slowly lowered by natural generation of acid end-productsas opposed to being quickly dropped by rapid addition of HCl togrowing cultures (1, 3, 4, 24). In batch culture, exposureof log-phase cells to a mild or moderately acidic pH (5.0 to 6.0)for 2 h resulted in enhanced survival of a significant proportionof the cell population upon exposure to the lower pH of 3.0 to3.5 (58). Although these in vitro conditions are extreme, theyprovide a convenient assay for distinguishing between unadaptedand adapted cells. De novo synthesis of proteins is required forthe enhanced survival of S. mutans log-phase cells at the lowpH (25, 59). This pH-inducible, growth phase- and time-dependentacid resistance has been well characterized in a number of bacteria;it is called the adaptive acid tolerance response (ATR) (18,20). Although many of the molecular mechanisms of the ATR inS. mutans remain unclear, a signal pH that results in sublethaleffects on the cells for sufficient time to allow synthesis ofprotective proteins appears to be important for induction of theATR.

In addition to responses to physical and chemical stresses, bacteria are known to regulate diverse physiological processesin a cell density-dependent manner, where secretion of an autoinducer(AI) is detected by neighboring cells that respond by activationof regulons that result in a variety of phenotypic changes (15).Examples include the initiation of bioluminescence in Vibrio fischeri(17), competence development in Streptococcus sp. (37, 41)and Bacillus subtilis (13), biofilm differentiation in Pseudomonasspp. (11, 48), bacteriocin production in Lactococcus spp.(31), conjugal plasmid transfer in Enterococcus faecalis (14),induction of virulence factors in Staphylococcus aureus (30),and stress responses in Escherichia coli (42). Cell density-dependentregulation in these systems appears to follow a common theme,in which a small, self-generated molecule is exported as the signalfor intercellular communication, commonly called quorum sensing(14). The best-characterized AIs in gram-positive bacteria aresmall peptides while in gram-negative bacteria the AIs are typicallyacylated homoserine lactones. Notably, genomic analyses have recentlyrevealed potential peptide signaling systems that may play a rolein cell-cell signaling in gram-negative bacteria (45).

During adherent growth, bacteria can sense their population size via quorum sensing and regulate gene expression and cellularfunctions as they adopt a biofilm phenotype (49). The changesin physiology and extracellular organization associated with thisresponse have often been equated to multicellular behavior andorganization in higher organisms (57). The ability of bacteriato communicate with one another by quorum sensing and behave collectivelyas a group can provide significant benefits in colonizing a newhost, defense against competitors and deleterious environments,cellular differentiation, and species evolution (12).

It is widely accepted that bacteria living in biofilms are more resistant to mechanical, physical, and chemical stresses (9,32, 48). Since S. mutans normally resides in a biofilm, theability to withstand acid in this physiological state is likelyan important adaptive response. The question of whether acid adaptationinvolves cell density-dependent events or cell-cell signalingin biofilms has not yet been addressed. Yet, in other bacteriait has been documented that the changes in external pH can significantlyinfluence many physiological parameters, such as energy coupling,ion transport, proton movement, and export of metabolic products,thereby triggering numerous secondary signals (35, 47). InE. coli and Salmonella spp., such signals activate one or moreglobal regulons that modulate expression of multiple gene operonsrequired for acid adaptation (18, 28). Furthermore, duringgrowth at pH 5.0, E. coli can signal acid tolerance to other unadaptedcells by secreting a protein-like molecule, termed extracellularinduction component (EIC) (54, 55). Although the signal moleculeremains unidentified, induction of acid adaptation in E. colipresumably involves cell-cellcommunication.

We have recently characterized a quorum sensing system in S. mutans that utilizes a 21-amino-acid competence stimulating peptide(CSP) that functions in the induction of genetic competence duringgrowth in biofilms (41). The system is typical of peptide pheromonesignal systems in streptococci and involves comC, comD, and comEgenes that, respectively, encode the precursor to the CSP, a histidinekinase and a response regulator. This is the first example ofa discrete cell-cell signaling mechanism that functions in biofilmsof gram-positive bacteria. Since we previously demonstrated thatcell-cell signaling via this system elicits phenotypic changesduring S. mutans biofilm growth, we initiated the present studyto examine the ATR of S. mutans biofilm cells and to determinethe effect of cell density on the ability of S. mutans to survivelow pH. We also assessed the ability of the CSP to enhance acidtolerance in both wild-type cells and defined mutants defectivein CSP production and tested culture filtrates collected fromlow-pH grown cultures for the ability to confer an acid-tolerantphenotype to unadaptedcells.

	MATERIALS AND METHODS

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Bacterial strains and growth media. All strains used in this study and their relevant characteristics are listed in Table 1. S. mutans BM71 (wild type) cellswere subcultured on Todd-Hewitt agar plates supplemented with0.3% yeast extract (THYE); the mutants were maintained on THYEagar containing 10 µg of erythromycin/ml. The medium used forassaying acid adaptation in batch cultures was tryptone (1%) yeastextract (0.5%) supplemented with 20 mM glucose (TYG) and 40 mMpotassium phosphate/citric acid at desired pH values. For continuouscultures, TYG medium was diluted 4× and supplemented with 0.01%hog gastric mucin (type III; Sigma). In some experiments, glucosein the medium was replaced by an equivalent concentration of sucroseto determine the effect of extracellular polysaccharide on acidtolerance of biofilm cells.

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TABLE 1. Bacterial strains and plasmid used in the study

We previously demonstrated the presence of the comCDE locus, the genes encoding a quorum sensing system, in six S. mutansstrains, including strain BM71 (41). We also used two strategiesto construct mutants of comC (SMCC1), comD (SMCD1), and comE (SMCE1)in S. mutans wild-type strain NG8. The same strategy was employedin this study to construct mutants defective in the same genesin S. mutans strain BM71 (41). To make the comC mutant SMCC-L1,we transformed pComC-KO plasmid DNA (pCR-Script harboring an inactivatedcomC gene; Amp^r, Em^r) into S. mutans BM71 after the plasmid was linearized by ScaIdigestion to disrupt the beta-lactamase gene. Transformed colonieswere selected on THYE-erythromycin (10 µg/ml) agar plates andthen confirmed by a rapid PCR protocol using the existing primersand strategy as described previously (41). The knockout mutantsof comD and comE were, respectively, generated by transformingpComD-KO (pVA8912 harboring a 292-bp internal comD fragment; Em^r) and pComE-KO (pVA8912 harboring a 462-bp internal comE fragment;Em^r) into S. mutans wild-type strain BM71. Chromosomal DNA was isolatedfrom transformants selected on THYE-erythromycin (10 µg/ml) agarplates to determine the presence of the erm gene at the desiredloci by PCR and Southern hybridization as previously described(41). The results confirmed inactivation of the comC, comD,and comE genes with the resultant mutants designated SMCC-L1,SMCD-L1, and SMCE-L1, respectively. Transformation assays (41)demonstrated that all three mutant strains were defective in geneticcompetence when compared with the parent strain BM71. Geneticcompetence was restored in strain SMCC-L1 by exogenous additionof theCSP.

Assay for acid adaptation in planktonic batch cultures. To facilitate measurement of acid adaptation in biofilm cells, S. mutans BM71 cells were first grown in batch culture to assaythe innate acid tolerance response in standard log- and stationary-phasecells by using a modification of methods described previously(33, 58). Mid-log-phase cells were obtained by transferringone volume of overnight culture into nine volumes (1:10) of freshTYG (pH 7.5) and incubated at 37^°C in an atmosphere of 5% CO₂ for 2 h. These cells were then collectedby centrifugation at 8,000 × g for 10 min and resuspended in 2ml of fresh TYG (pH 5.5) at various cell densities as determinedby the optical density at 600 nm (OD₆₀₀). The cells were inducedfor acid adaptation by incubation at a "signal pH" of 5.5 for1 to 3 h at 37^°C with 5% CO₂. The adapted log-phase cells were then exposed tothe killing pH, which was predetermined by incubating unadapted,mid-log phase cells in TYG medium at pHs from 6.0 to 2.0 for 3h. Stationary-phase cells were prepared by resuspending late-logphase cells in TY medium (tryptone-yeast extract) without glucose.The culture was incubated at 37^°C for 2 h to allow the cells to enter stationary phase. Inductionof acid adaptation in stationary-phase cells followed a similarprocedure to that for log-phase cells except that glucose wasomitted. Adaptation of both log- and stationary-phase cells toacidic pH was determined by measuring the ability of the bacteriato survive a killing pH for 3 h. Acid killing was initiated byresuspending cells in the same volume of fresh TYG medium (pH3.5), and an aliquot of cell suspension was taken immediatelyfrom each sample to determine the total viable-cell number attime zero. The cells were then incubated for 3 h at 37^°C with 5% CO₂, and aliquots were taken at various times to determinethe percent survival by viable cellcounts.

Acid adaptation of S. mutans biofilms grown in continuous culture. S. mutans BM71 cells were grown in a chemostat-based continuous flow fermentor for the development of biofilms as previouslydescribed (39, 41). Adaptation of biofilm cells to low pHwas induced directly in the chemostat by pulsing 40 mM glucoseinto steady-state cultures and disconnecting the pH control. Theculture pH was allowed to drop by the accumulation of acid end-productsgenerated from glucose metabolism. The growth of bacterial cellsunder this condition was limited by glucose, as determined byassaying residual glucose in the cultures. Initial experimentsshowed that following the glucose pulse without pH control ata dilution rate of 0.1 h¹, the culture pH dropped rapidly to around pH 5.5 in the first40 min. The pH continued to decrease for about 6 h until reachingits lowest point of pH 4.92. The pH remained at this level forabout 1 to 2 h and slowly returned to about pH 5.95. Adaptationof the cultures was allowed to occur for at least one mean generationtime (6.93 h at a dilution rate [D] of 0.1 h¹). Samples were then taken from both the biofilms and the planktonicphase to assess survival of bacterial cells to the killing pH.Control samples (unadapted cells) were also taken from a duplicateculture under pH control (at a constant pH of 7.0) following glucosepulse.

Acid killing of biofilm cells. Biofilms on glass rods were removed from the chemostat and divided into two groups for acid killing experiments: one groupof biofilms was dissociated from the surfaces (dispersed biofilms),and the other group remained attached to the surfaces (intactbiofilms). Dissociation of biofilms from surfaces was performedby sonication using the BioSonik IV (Bronwill, Rochester, N.Y.)with a low power output at a setting of 20 for 20 s. This procedureremoved >99% of the attached cells as estimated by comparing platecounts and scanning electron micrographs (41). The procedureresulted in dispersion of the majority of aggregates and disruptionof chains into single cells, as indicated by light microscopy.Aliquots (200 µl) of the cell suspension were taken from the dissociatedbiofilm samples to determine the viable cell number at time zero.Total cell numbers in intact biofilms were determined by growingeight rods under identical conditions and using four rods forenumeration following sonication and four rods for the acid killingexperiments. Biofilm cells dispersed from, or intact on, eachrod were suspended in 2 ml of fresh TYG (pH 3.5) in a 5-ml glasstube and incubated at 37^°C with 5% CO₂ for 3 h. Following acid killing, intact biofilmswere dissociated from the surface by sonication. All samples wereserially diluted in 10 mM potassium phosphate buffer (pH 7.2)and plated on THYE agar plates by using a spiral plater (modelD; Spiral System Inc., Cincinnati, Ohio). The number of survivingcells was determined by counting colonies after the plates wereincubated at 37^°C with 5% CO₂ for 2 to 3 days. Percent survival was expressedas the number of viable cells after acid killing over the totalnumber of viable cells at time zero when cells were exposed tokilling pH (3.5).

Preparation of culture filtrates and induction of acid adaptation. To determine if low-pH growing cultures contained EICs capable of inducing an ATR, cell-free supernatants were prepared fromchemostat cultures of S. mutans wild-type strain BM71 and thecomC mutant (SMCC-L1) grown in undiluted TYG medium (3% tryptone,1% yeast extract, and 20 mM glucose). Cell-free supernatants werecollected from chemostat cultures at a dilution rate (D) of 0.2h¹ at 4 h after a pulse of 40 mM glucose with or without pH control.The cell-free supernatant collected from the culture without pHcontrol (pH 5.2 ± 0.3 [mean ± standard deviation {SD}]) was neutralizedto pH 7.0 with KOH and sterilized by passage through a 0.2-µm-pore-sizefilter (Millipore, Bedford, Mass.), whereas the supernatant collectedfrom the culture with pH control (pH 7.0) was filter sterilizedwithout adjustment of pH. All culture filtrates were then keptat $-$ 20^°C until use. Some samples were treated either with heat (65^°C) for 30 min or with proteinase K (37^°C) for 1 h before addition to the cultures. Before their use forinduction of the ATR, culture filtrates were added to an equalvolume of fresh TYG (pH 7.5) to provide the cells with an energysource. Induction of acid adaptation was initiated by incubatinglog-phase cells with the culture filtrates for 2 h before exposingthem to the killing pH. The effect of culture filtrate concentrationon acid adaptation was determined by diluting the filtrates one-to eightfold inTYG.

Acid adaptation in comC, comD, and comE mutants. The comCDE operon encodes a quorum sensing system that controls the cell density-dependent induction of genetic competencein S. mutans (41). We examined the effects of inactivation ofthe comC, comD, and comE genes on acid adaptation in S. mutans.Assays for ATR in the mutants were performed by the same methodsdescribed above. In addition, we used a 21-amino-acid syntheticsignal peptide deduced from the comC gene sequence (41) to determineif the CSP restored acid tolerance in the comC mutant during acidadaptation. The CSP was freshly dissolved in sterile distilledwater to a concentration of 1 mg/ml. The solution was then addedto the cultures at a final concentration of 2 µg/ml 2 h afterinoculation of cells. To determine if secondary signals couldaugment the activity of the CSP, the pH-adjusted culture filtratesfrom acid adapted cultures of the comC mutant were used to assayATR in conjunction with the CSP as describedabove.

Scanning electron microscopy. To examine the spatial distribution and biofilm density by scanning electron microscopy, biofilms of different ages were removed,washed once with 10 mM KPO₄, and fixed with 2 ml of 3.7% formaldehydein 10 mM KPO₄ buffer overnight. The samples were then dehydratedwith a series of alcohol washes (30, 50, 70, 95, and 100%), criticalpoint dried with liquid CO₂, mounted, and sputter-coated withgold. The samples were then examined using a scanning electronmicroscope (model S-2500; Hitachi Instruments, San Jose, Calif.).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

pH limit for survival. To assess the ATR, the pH limit for survival of S. mutans BM71 was first determined by measuring viability after exposureof mid-log phase cells to media at pHs from 2.0 to 6.0 for 3 h.S. mutans BM71 cells grew and maintained 100% viability at pH6.0 to 5.5, and the cells still survived well at pH 5.0 (91 to98%). At lower pH, the survival rates rapidly decreased, with100% of the cells killed after exposure to pH 3.0. Since exposureto pH 3.5 for 3 h could kill over 99.99% of unadapted log-phasecells, we used this pH as the killing pH to assess the ATR inthisstudy.

Cell density modulates induction of acid adaptation. The ability of S. mutans to tolerate exposure to pH 3.5 via pH-induced ATR in log-phase cells was modulated by the populationdensity (Fig. 1). At the higher cell densities (OD₆₀₀ of 0.6 orhigher, approximately 10⁹ cells/ml or more), S. mutans BM71 cells rapidly became adaptedto low pH; the induction of adaptation was optimal after 2 h ofincubation at pH 5.5 (Fig. 2). Additional exposure (3 h in total)to this signal pH did not further enhance survival of cells toacid challenge. Induction of ATR in log-phase cells at a low celldensity (0.2 at OD₆₀₀, or 10⁶ cells/ml) by exposure to the signal pH for 2 h was insufficientfor optimal development of acid adaptation. Increasing the inductiontime further enhanced acid adaptation, although the magnitudeof acid resistance at the low cell density was still lower thanthat observed with the higher cell density (Fig. 2). In this study,we used the cell density of 0.6 at OD₆₀₀ for most experimentsunless specified. To test whether increased cell density was specificto the adaptation phase, we performed an additional experimentin which S. mutans cells were induced for acid adaptation at pH5.5 for 2 h at a high density (0.6 at OD₆₀₀) and then dilutedto OD₆₀₀'s of 0.1 and 0.2. These diluted cells and the undilutedsample were exposed to pH 3.5 for 3 h. The results demonstratedthat there was no statistical difference in the percentage ofsurvival found between the different groups with T-test (P valueof 0.05) (data not shown).

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FIG. 1. Effect of cell density on induction of acid adaptation in S. mutans BM71 log-phase cells. Cells were collected from pH 7.0 cultures and resuspended at various cell densities during the adaptation phase at pH 5.5 for 2 h and were then exposed to the killing pH of 3.5 for 3 h. Results are the mean ± SD of at least three independent cultures.

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FIG. 2. Effects of cell density and adaptation time on induction of acid adaptation by S. mutans BM71. Cells were adapted by incubation in pH 5.5 TYG medium at low (OD₆₀₀ = 0.2) or high (OD₆₀₀ = 0.6) density for various times before exposure to the killing pH of 3.5 for 3 h. Results represent the mean number of surviving cells ± SD from at least three independent cultures.

S. mutans BM71 exhibits both log- and stationary-phase ATR. We tested the ATR of planktonic cells in log and stationary phase for comparison to biofilm-grown cells. The results frombatch cultures indicated that survival of S. mutans BM71 to killingpH involved at least two adaptive systems that were dependentof growth phase (Fig. 3). The first system appeared during logphase growth in which preexposure of cells to pH 5.5 for 2 h protectedthe cells against subsequent killing at pH 3.5. The adapted log-phasecells survived approximately 50- to 100-fold better than the unadaptedcells following exposure to the killing pH for 3 h.

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FIG. 3. Survival kinetics of S. mutans BM71 exposed to killing pH of 3.5. Both adapted and unadapted stationary- and log-phase cultures were sampled at various time points after exposure to the killing pH of 3.5. The number of survivors was determined from at least three independent cultures.

Acid protection was also induced by entry into carbon starvation-induced-stationary phase by incubation in medium devoid ofglucose as described. These stationary-phase cells had an equivalentor slightly increased resistance to the killing pH 3.5 than thelog-phase pH-induced cells (Fig. 3). Further exposure of stationary-phasecells to pH 5.5 for 2 h only slightly enhanced resistance to thekillingpH.

Culture filtrate induces log-phase ATR. The observation that high cell density promoted induction of acid adaptation (Fig. 1), suggested that S. mutans BM71, duringexposure to a low (signal) pH, utilizes a cell density-dependentmechanism to enhance induction of acid adaptation in the populationvia release of an extracellular signal molecule(s). To test thishypothesis, we collected cell-free supernatants from S. mutanschemostat cultures grown at low pH (5.2 ± 0.3) and assayed acidadaptation conferred by neutralized culture filtrate, as describedin Materials and Methods. After incubation in the neutralizedculture filtrate for 2 h, log-phase cells of S. mutans BM71 becamemore resistant to the killing pH than cells incubated in the filtratecollected from the culture at pH 7.0 (Fig. 4). Dilution of theculture filtrate with fresh TYG (pH 7.5) resulted in a titratabledecrease in acid resistance, demonstrating that the acid adaptationwas dependent on the concentration of the culture filtrate and,consequently, EICs. The culture filtrates at dilution factorsof 1:1 and 1:2 revealed no significant difference in the effecton induction of acid adaptation. This suggested that the culturefiltrates at both dilutions might represent a saturated concentrationof the EIC required for acid adaptation. The EIC(s) in the culturefiltrate were probably proteinaceous since heat or proteinasetreatment abolished their effect on induction of acid adaptation(Fig. 5).

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FIG. 4. The neutralized culture filtrate collected from the chemostat at pH 5.2 ± 0.3 (mean ± standard deviation) was able to induce a log-phase ATR. The culture filtrate was diluted with fresh TYG medium (pH 7.5) to illustrate a dose-dependent effect. The results are the mean ± SD of at least three independent cultures.

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FIG. 5. Effect of heat or proteinase treatment on induction of acid adaptation in S. mutans BM71 by pH-neutralized culture filtrates collected from pH 5.2 (adapted) and pH 7.0 (unadapted) cultures. The results are the mean ± SD of at least three independent cultures.

Inactivation of comCDE genes results in reduced log-phase ATR. Since the S. mutans comCDE operon encodes a peptide pheromone quorum sensing system that controls the cell density-dependentcompetence phenotype in S. mutans biofilms (41), we examinedthe ability of mutants with defects in the signaling system towithstand acid challenge. Disruption of the comC, comD, or comEgenes resulted in a diminished log-phase ATR (Fig. 6). Even afterexposure to adaptive pH for 2 h, the mutants were still 10-foldmore sensitive to the killing pH than the wild-type strain. However,unadapted mutants did not show substantial defects in their ATRrelative to the parent strain BM71. Addition of CSP to the cultureof the comC mutant during acid adaptation partially restored thewild-type ATR. These results demonstrated that the quorum sensingsystem plays a role in induction of acid adaptation.

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FIG. 6. Acid tolerance was assayed in mutants defective in comC, comD, and comE, the genes encoding a quorum sensing system essential for cell density-dependent induction of genetic competence in unadapted and adapted S. mutans log-phase grown cells. Addition of CSP into the culture of comC mutant partially restored the wild-type acid tolerance. The results are the mean ± SD of four independent cultures.

To further test for the presence of secondary molecules that augment the ATR mediated by the signal peptide, we tested thecell-free culture supernatants collected from the comC mutantfor their ability to enhance the ATR in the comC mutant in theabsence or presence of exogenous CSP. The pH-adjusted culturefiltrate from the comC mutant plus the synthetic CSP almost completelyrestored the log-phase ATR, whereas the CSP or the culture filtratealone only partially restored the ATR (Fig. 7). The results suggestedthe presence of a second signal molecule(s) in S. mutans culturesupernatant that could augment the ATR.

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FIG. 7. The pH-adjusted culture filtrates collected from comC mutant (SMCC-L1) cultures that were maintained at pH 7.0 (filtrate 1) or pH 5.2 (filtrate 2) were added either individually or with synthetic CSP to unadapted SMCC-L1 cultures before exposure to the killing pH 3.5 for 3 h. The percentage of survivors ± SD was determined from four independent cultures.

Physical characteristics of biofilms formed in chemostat. To induce acid adaptation in biofilm cells without disrupting the biofilm architecture, we used a chemostat-based biofilmfermentor to establish acid adaptation via acid generated fromglucose metabolism of the cells. The cell density of S. mutansbiofilms grown under glucose limitation, in terms of total biomass,biofilm thickness, and number of viable cells, is a function ofthe accumulation time (38). The relative cell densities of biofilms,as represented by the number of viable cells, after glucose pulsewith or without pH control are shown in Table 2. Generally, thedensity of S. mutans BM71 biofilms increased with accumulationtime and glucose availability, with or without pH control. Interestingly,the cell number in the biofilms after glucose pulse but withoutpH control was about twofold higher than that of biofilms grownunder pH control. Conversely, the yield of planktonic cells presentafter the natural pH drop ([8.4 ± 2.8] × 10⁷CFU/ml) was lower than that with pH control ([27.6 ± 6.4] × 10⁷CFU/ml). The results suggested that active multiplication of theplanktonic cells after a glucose pulse without pH control wasrapidly reduced or even arrested by the acid generated from theculture. In contrast, the biofilms continued to accumulate onthe surface during the pH shift, resulting in a three- to fivefoldincrease in the number of viable cells. When cultures were pulsedwith sucrose, S. mutans BM71 cells formed even thicker and denserbiofilms than with glucose; extracellular polysaccharide was clearlyvisible with scanning electron microscopy (data not shown).

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TABLE 2. Viable cell numbers of S. mutans (BM71) biofilms grown at D of 0.1 h¹ following 40 mM glucose pulse with or without pH control

Acid tolerance of biofilm-grown cells. To determine the effects of biofilm integrity on the ability of the cells to withstand acid stress, we compared acid toleranceof S. mutans in both intact and disrupted biofilms. Disruptionof structural integrity showed little effect on acid resistanceof biofilms grown with glucose as a carbon source (Fig. 8). However,the thicker, intact biofilms formed in sucrose-containing mediumshowed three- to fivefold more resistance to killing pH than theresuspended biofilm cells (Fig. 8), demonstrating that extracellularpolysaccharide enhanced acid resistance of bacteria within biofilms.To minimize the difference in cell numbers in biofilm-grown cellsfor acid killing experiments, we resuspended the dispersed biofilm-growncells in TYG medium to a cell density of 0.6 at OD₆₀₀ prior toexposure to the killing pH. The results indicated that the developmentof acid adaptation in actively growing biofilms varied with thecell density or thickness of the biofilms regardless of whetherthe films were dispersed or left intact. Cells from the thickerand denser biofilms had a much higher resistance to the killingpH than the planktonic cells and adapted log-phase cells (Fig.9). For example, cells recovered from 5-day biofilms that containedthe highest cell density per unit area (over 10⁸/cm²) were about 30-fold more resistant to the killing pH than theplanktonic cells or even the 12- to 24-h biofilms. The resultsprovided further evidence that biofilms with high cell densityfacilitated induction of acid adaptation in S. mutans.

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FIG. 8. Effect of biofilm integrity on acid resistance of biofilms. Biofilms were either intact or dissociated from the surfaces by sonication. The biofilms were grown under the condition of either glucose or sucrose as a carbon source as described in Materials and Methods.

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FIG. 9. Acid tolerance response of S. mutans BM71 biofilm cells. LPC, log-phase cells; PLC, planktonic cells; 12HB, 12-h biofilm; 1DB, 1-day biofilm; 5DB, 5-day biofilms. Results are the means ± standard deviation of four cultures.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Since dental caries develops in an intermittently acidic environment, one of the most significant virulence properties ofcariogenic bacteria like S. mutans is their acid tolerance. Underhigh-carbohydrate conditions, S. mutans outcompetes some of themost acidogenic and aciduric species in dental plaque (3, 5,7). The evidence from these studies suggests that inductionof acid adaptation in S. mutans is an important virulence factorsince its aciduricidy is a feature that sets it apart from a numberof other oral bacteria (58). Adaptation of S. mutans to lowpH in its natural ecosystem of dental plaque is usually characterizedby active transport of carbohydrates, increased glycolytic activity,and an increase in cell number (7, 10, 23, 27, 46).

In planktonic culture, exposure of S. mutans to an extracellular signal pH between 5.5 and 5.0 results in the synthesis ofa subset of proteins that enhances its ability to survive low-pHchallenges (25, 59). The molecular mechanisms of the S. mutansATR remain poorly understood, especially during growth in biofilms,where the cells are known to exhibit a phenotype different fromthat of planktonic cells. Since S. mutans normally encountersacid while living in dense biofilm communities, we proposed thathigh cell densities of S. mutans may facilitate its survival againstlow-pH challenges. Testing this hypothesis led us to the unprecedentedfinding that the ATR interfaces with a density-dependent signalingpathway that also initiates geneticcompetence.

Since S. mutans relies on a biofilm lifestyle for survival and utilizes a quorum sensing system to modulate genetic competencevia a cell density-dependent mechanism (41), we set forth toinvestigate a possible connection between cell density, biofilmgrowth, and quorum sensing in the process of acid adaptation byS. mutans. Our results clearly showed that cell density modulatedacid adaptation in S. mutans log-phase cells, since S. mutansgrown at high cell density established adaptation to the signalpH more rapidly than the cells at the lower density. Similarly,S. mutans cells grown in a high cell density biofilm were moreresistant to the killing pH than planktonic-phase cells. In fact,S. mutans cells grown in biofilms not only survived better thanthe planktonic cells but were also capable of growth at the lowerpH following a glucose pulse (Table 2). It is likely that optimalinduction of acid adaptation in a population of S. mutans requiresa coordinated activity through mechanisms involving both low pHinduction and cell density-dependent intercellularcommunication.

Based on the evidence obtained from this study, we propose that S. mutans, upon exposure to low pH in a growing culture, releasesan extracellular signal molecule(s) to enhance induction of acidadaptation in the population. The evidence that neutralized culturefiltrates prepared from acid-adapted cells induced a log-phaseATR in cells that had never encountered the signal pH and thatthe extent of the acid tolerance varied with cell density andconcentration (titration) of the culture filtrate strongly supportsthis hypothesis. The EIC(s) produced during acid adaptation probablyacted as a secondary signal to amplify the induction of acid adaptationin the population. Upon detection of falling pH this signal islikely secreted and detected by neighboring cells to activatethe ATR to protect them from the impending pH drop, caused bysugar metabolism. In addition, our preliminary results indicatedthat the extracellular component(s) in the culture filtrate responsiblefor the induction of acid adaptation were protein-likemolecule(s).

We have recently identified and characterized a peptide-mediated quorum sensing system essential for the cell density-dependentinduction of genetic competence in S. mutans (41). Since thisquorum sensing system functions optimally during biofilm growth,we investigated the role that this system plays in the inductionof acid adaptation. This quorum sensing system consists of atleast five gene products, including a 21-amino-acid CSP (aminoacid sequence, SGSLSTFFRLFNRSFTQALGK) whose precursor is encodedby comC, a histidine kinase sensor protein encoded by comD, andthe cognate response regulator encoded by comE. The comCDE genesare located in the same locus and together constitute a signalsensing system for generating and responding to the active CSP.Two other genes required for peptide processing and export, cslAB(comAB), are located on a separate region of the chromosome andencode a CSP-specific secretion system consisting of an ATP-bindingcassette transporter cslA (ComA) and its accessory protein cslB(ComB) (50; J. H. Lee, P. C. Y. Lau, Y.-H. Li, M. Meloche, A.J. Cuttichia, R. P. Ellen, and D. G. Cvitkovitch, submitted forpublication). Our previous experiments demonstrated that thiscell-cell signaling system produced optimal genetic competencewhen the cells were living in actively growing biofilms. In thepresent study, we found a connection between the competence signalingpathway and the ATR, suggesting that the CSP may function as anEIC.

The results clearly showed that mutants defective in the comC, comD, or comE genes had a diminished log-phase ATR, althoughcells exposed to the signal pH still remained more resistant tothe killing pH than unadapted cells, suggesting that inductionof acid adaptation in S. mutans is regulated by more than onesystem or signal. To test if a second secreted signal moleculewas involved, we collected the cell-free culture supernatantsfrom cultures of acid adapted and unadapted comC mutant SMCC-L1(unable to produce the CSP) and assayed for the ability of thepH-neutralized filtrate to enhance the ATR in unadapted SMCC-L1in the presence or absence of exogenous CSP. The results demonstratedthat the pH-adjusted culture filtrate collected from the adaptedcomC mutant did contain a signal molecule(s) that contributedto the overall ATR. In fact, addition of both the pH-adjustedculture filtrate and the synthetic CSP almost completely restoredthe log-phase ATR in SMCC-L1, demonstrating that CSP and at leastone other signal molecule present in the S. mutans culture supernatantcontribute to induction of theATR.

This study also demonstrated that S. mutans BM71 was able to survive low-pH challenge after exposure to a signal pH of 5.5and was modulated by cell density. This result was consistentwith the findings of Svensäter et al. (59), who demonstratedthat exposure of log-phase S. mutans to the signal pH (5.0 to5.5) up-regulated the synthesis of 64 proteins, 25 of them acidspecific, although 49 proteins exhibited diminished synthesisupon low-pH exposure. Preliminary studies with S. mutans strainNG8 demonstrated, by comparison of two-dimensional (2-D) gel profiles,that at least 10 identical proteins were induced by both low pHand by the CSP (data not shown). To further support the hypothesisthat EIC(s) were involved and we were not simply observing a phenomenonresulting from cells forming physical aggregates, the acid shockat pH 3.5 was repeated with cells at various densities, and nodifference in percent survival wasobserved.

Acid tolerance was also enhanced during stationary phase brought about by carbon starvation. These conditions provided thecells with an equivalent or even slightly higher level of acidresistance than the log-phase ATR. A similar result was observedby Svensäter et al. (59), who showed that carbon starvationin S. mutans resulted in a 7- to 12-fold increase in the resistanceto acid killing when compared with the cells grown in medium with20 mM glucose. More recently, Zhu et al. (60) reported thatstarvation induced by resuspending S. mutans cells in 40 mM phosphatebuffer (pH 7.0) for 24 h resulted in a significant increase insurvival of both biofilm and planktonic cells to killing by lacticacid (pH 3.8). In Salmonella spp. and E. coli, this stationaryphase acid tolerance system is part of a general stress resistanceinduced by entry into stationary phase and regulated by an alternativesigma factor, RpoS (18, 36). The system provides cross-protectionagainst a number of other stresses, such as heat, cold, oxidation,high osmolarity, and heavy metals (18, 19, 28). A similargeneral stress resistance has been identified in several gram-positivebacteria, including Lactococcus lactis (53), Lactobacillus acidophilus(56), and B. subtilis (51), although the molecular mechanismcontrolling the general stress resistance in gram-positive bacteriaremains unclear. We anticipate that starvation-induced acid resistancein S. mutans represents the same general stress resistance observedin other gram-positive organisms. The stationary phase stressresistance mechanism is likely very important for the survivalof S. mutans in biofilms since it is believed that the biofilmphenotype is akin to the physiological state that cells existwhen in stationary phase (60).

It has been widely reported that bacteria grown as a surface biofilm are more resistant to various stress challenges and antimicrobialagents than planktonic cells (9). The results from our presentwork and other studies demonstrated that S. mutans grown as abiofilm is more resistant to low-pH challenge than the cells insuspension (60). The underlying mechanisms that lead to increasedresistance of biofilms to stress are not well understood. It wasoriginally believed that the increase in resistance was providedto bacterial cells by the physical barrier that exists withinbiofilms, resulting in diffusion-limiting gradients (8). WithS. mutans, however, the physical barrier of biofilms appears toplay a limited role in acid diffusion, since use of a proper bufferingsystem in liquid phase provides a relatively good control of biofilmpH, as shown by monitoring the in situ pH of biofilms in an invitro experimental system (6, 40). Biofilms grown in aquaticenvironments usually form a 3-D, mushroom-like structure withnumerous water channels within the biofilms, which allow variousions and small molecules to diffuse throughout the biofilms (9,49). The data from this study also showed that intact biofilmsgrown with glucose as a carbon source did not provide significantphysical protection against lethal acid, since cells that wereremoved from biofilms and were dispersed and resuspended in mediumwere equally resistant to acid stress, as were cells in intactbiofilms. This suggests that the increased acid resistance observedwith S. mutans biofilm cells probably resulted from changes inthe cells' physiology, mediated in part by extracellular signalmolecules. When sucrose was added to the biofilm cultures, therewas a marked increase in acid resistance. It is likely that thisarises partly from the altered biofilm architecture resultingfrom accumulation of extracellular polysaccharide formed undertheseconditions.

Biofilms, particularly thicker biofilms, may provide bacterial cells with a unique environment to fully express their adaptivesurvival mechanisms. Because of 3-D structures, high cell density,and diffusion barriers, bacterial cells at different locationswithin a biofilm may not sense the same degree of pH stress simultaneously.The cells that first sense a pH stress may rapidly process theinformation and pass their secondary signal to the other membersof the population through cell-cell signaling systems to initiatea coordinated protective response against potentially lethal acid.Unlike planktonic cells that need to reach a critical concentrationof signal molecules and cell density, biofilms can allow signalmolecules to accumulate rapidly in the local environment to initiatecoordinated activities far more quickly (44, 49). In addition,physiological states of bacterial cells living in a biofilm, interms of growth rate, growth phase, or metabolic activities, areheterogeneous. This allows the cells to respond to stress in differentways. Apparently, a biofilm population has several advantagessince the cells have more time, a sufficient concentration ofsignal molecules, and high population density to adapt to stressrelative to planktoniccells.

We conclude that the ATR in S. mutans has both a log-phase ATR and a general acid resistance system in stationary-phase cells.Population density and cell-cell signaling modulate acid adaptationin S. mutans log-phase cells. Since S. mutans cells grown in high-cell-densitybiofilms were invariably more resistant to the killing pH thanthe planktonic cells, we propose that high-cell-density biofilmsprovide a unique environment for induction of acid adaptationvia quorum sensing in S. mutans. The quorum sensing pathway significantfor the ATR intersects the regulatory pathway for genetic competence.It is likely that the biofilm growth mode allows S. mutans toutilize multiple mechanisms for survival during low pH stress,and these are dependent on carbohydrate availability, externalpH, growth phase, population density, and various coordinatedactivities.

	ACKNOWLEDGMENTS

We thank Marie-Christine Kean for help in preparation of themanuscript.

Our work was supported by PHS grant DE 013230-01 from the National Institute of Dental and Craniofacial Research and grantMT-15431 from the Medical Research Council of Canada and by infrastructuregrants from the Canadian Foundation for Innovation and The OntarioInnovation Trust. D.G.C. is supported by a Canada Research Chairand M.N.H. is the recipient of a University of Toronto Open Fellowshipand Ontario Graduate Scholarship in Science andTechnology.

	FOOTNOTES

^* Corresponding author. Mailing address: Rm. 449A, Dental Research Institute, University of Toronto, 124 Edward St., Toronto,Ontario M5G 1G6, Canada. Phone: (416) 979-4917, ext. 4592. Fax:(416) 979-4936. E-mail: dennis.cvitkovitch{at}utoronto.ca.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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