Defects in D-Alanyl-Lipoteichoic Acid Synthesis in Streptococcus mutans Results in Acid Sensitivity

doi:10.1128/JB.182.21.6055-6065.2000

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Journal of Bacteriology, November 2000, p. 6055-6065, Vol. 182, No. 21
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Defects in D-Alanyl-Lipoteichoic Acid Synthesis in Streptococcus mutans Results in Acid Sensitivity

David A. Boyd,¹ Dennis G. Cvitkovitch,²^,³ Arnold S. Bleiweis,³ Michael Y. Kiriukhin,⁴ Dmitri V. Debabov,⁴ Francis C. Neuhaus,⁴ and Ian R. Hamilton¹^,^*

Department of Oral Biology, University of Manitoba, Winnipeg, Manitoba R3E 0W2,¹ and Dental Research Institute, Faculty of Dentistry, University of Toronto, Toronto, Ontario M5G 1G6,² Canada; Department of Oral Biology, University of Florida, Gainesville, Florida 32610³; and Department of Biochemistry, Molecular and Cell Biology, Northwestern University, Evanston, Illinois 60208⁴

Received 20 March 2000/Accepted 3 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

In the cariogenic organism, Streptococcus mutans, low pH induces an acid tolerance response (ATR). To identify acid-regulatedproteins comprising the ATR, transposon mutagenesis with the thermosensitiveplasmid pGh9:ISS1 was used to produce clones that were able togrow at neutral pH, but not in medium at pH 5.0. Sequence analysisof one mutant (IS1A) indicated that transposition had createda 6.3-kb deletion, one end of which was in dltB of the dlt operonencoding four proteins (DltA-DltD) involved in the synthesis ofD-alanyl-lipoteichoic acid. Inactivation of the dltC gene, encodingthe D-alanyl carrier protein (Dcp), resulted in the generationof the acid-sensitive mutant, BH97LC. Compared to the wild-typestrain, LT11, the mutant exhibited a threefold-longer doublingtime and a 33% lower growth yield. In addition, it was unableto initiate growth below pH 6.5 and unadapted cells were unableto survive a 3-h exposure in medium buffered at pH 3.5, whilea pH of 3.0 was required to kill the wild type in the same timeperiod. Also, induction of the ATR in BH97LC, as measured by thenumber of survivors at a pH killing unadapted cells, was 3 to4 orders of magnitude lower than that exhibited by the wild type.While the LTA of both strains contained a similar average numberof glycerolphosphate residues, permeabilized cells of BH97LC didnot incorporate D-[¹⁴C]alanine into this amphiphile. This defect was correlated withthe deficiency of Dcp. Chemical analysis of the LTA purified fromthe mutant confirmed the absence of D-alanine-esters. Electronmicrographs showed that BH97LC is characterized by unequal polarcaps and is devoid of a fibrous extracellular matrix present onthe surface of the wild-type cells. Proton permeability assaysrevealed that the mutant was more permeable to protons than thewild type. This observation suggests a mechanism for the lossof the characteristic acid tolerance response in S. mutans.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Lipoteichoic acids (LTAs) are surface components of most gram-positive bacteria comprised of phosphodiester-linked poly(alditolphosphate)chains covalently anchored to membrane glycolipid. The LTA ofmany oral streptococci is comprised of polyglycerolphosphate [poly(GroP)](30), with each GroP unit potentially glycosylated and selectivelyacylated with D-alanine ester residues (16). D-Alanyl estersof LTA have important functions in growth and physiology, includinga role in the synthesis of wall teichoic acid (34, 45), regulationof autolytic activity (16), and the binding of Mg²⁺ for enzyme activity (2). The polyanionic properties of LTAare associated with adherence and cell-cell coaggregation throughthe binding of cations (36), proteins and polysaccharides (14),as well as hydroxyapatite (9). These are important factorsin the formation of dental plaque biofilms. Streptococcus mutans,an organism associated with dental caries, synthesizes considerableLTA (25), particularly under the low growth rates typical ofthe plaque biofilm (7).

The biosynthesis of D-alanyl-LTA, studied in Lactobacillus rhamnosus (12, 27, 28, 42) and Bacillus subtilis (46),requires the D-alanyl-carrier protein (Dcp) for incorporationof the activated D-alanine into membrane-associated LTA (mLTA).The activation and ligation of D-alanine to Dcp is catalyzed byD-alanine:Dcp ligase (D-alanine-Dcl) having a function similarto the acid thiol ligases (28). Unlike the first reaction, thetransfer of activated D-alanine to mLTA is highly specific forD-alanine-Dcp. Recent genetic analysis (11, 42) has indicatedthat the proteins for D-alanine incorporation reside in the dltoperon comprised of four genes:dltA, encoding Dcl; dltC, encodingDcp; dltB, encoding a putative transmembrane protein involvedin the secretion of activated D-alanine; and dltD, a membrane-associatedthioesterase for mischarged carrierprotein.

Two recent reports have indicated that oral streptococci possess the dlt operon comprised of dltA, dltB, dltC, and dltD havinghomology to the operons of L. rhamnosus and B. subtilis. In onestudy, Spatafora et al. (49) observed that the inactivationof the S. mutans UA130 dlt by transposon insertion into a siteupstream of dltA resulted in the diminished synthesis of intracellularpolysaccharide. Interestingly, the expression of the dlt operonwas induced in the exponential phase when the cells were grownwith sugars transported by the phosphoenolpyruvate-sugar phosphotransferasesystem (PTS) but was expressed constitutively when grown withthe non-PTS sugars raffinose and melibiose. A mutant of S. mutansdefective in PTS activity showed constitutive expression, suggestinga relationship between the dlt operon and sugar transport viathe PTS. In a second study (10), insertional inactivation ofdltA in S. gordonii DL1 (Challis) not only resulted in the lossof D-alanylation of LTA, but also the loss of intrageneric coaggregationwith other oral streptococci. Such inactivation also resultedin the loss of a 100-kDa surface protein adhesin known to be associatedwith this aggregation. In spite of this defect, the mutant was,nevertheless, able to carry out intergeneric coaggregation withhuman oral actinomyces. It was postulated that the D-alanyl-LTA,but not D-alanine-free LTA, provided binding sites for the adhesinto facilitate intragenericcoaggregation.

In human dental plaque, S. mutans is subjected to daily cycles of acid shock created by the accumulation of acid end productsgenerated during the metabolism of dietary carbohydrate by theacidogenic microflora. The rate of acid formation in human subjects,as measured by pH telemetry, has indicated that the intake ofcarbohydrate can lower the plaque pH from 7.0 to 4.0 in as littleas 3 min (31, 32). Our earlier studies (24, 50, 51)demonstrated that the acid shock (pH 7.5 to 5.5) of log-phasecells of S. mutans resulted in the induction of an acid toleranceresponse (ATR) that enhanced survival at pH 3.0. This log-phaseATR requires protein synthesis and involved the transient formationof acid-responsive proteins over a 2-h period (24). This acidshock results in the upregulation of 64 proteins within 30 minof the pH change (51). These are undoubtedly related to thevariety of physiological changes induced in cells during pH downshiftsin continuous culture (21).

Our goal is to identify the key global regulators involved in the ATR in S. mutans. To this end, transposon mutagenesis hasbeen used to isolate clones that are acid sensitive. During thisprocess, an acid-sensitive clone was isolated carrying a 6.3-kbdeletion, which included dltA and a portion of dltB of the dltoperon as well as four complete genes upstream from that operon.To test whether the defect in the dlt operon was associated withthe acid-sensitive phenotype, the D-alanylation of LTA in S. mutansLT11, was blocked by the inactivation of dltC. The resulting mutant,BH97LC, exhibited enhanced acidsensitivity.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains, plasmids, and growth conditions. Bacterial strains and plasmids are listed in Table 1. S. mutans strains were maintained anaerobically at 37°C (or 30 or 42°Cwhen appropriate) on Todd-Hewitt plates (Difco or BBL) and grownfor DNA isolation in Todd-Hewitt broth supplemented with 0.3%yeast extract (THYE). For selection of acid-sensitive colonies,THYE plates containing 50 mM sodium acetate at pH 5.3 and pH 5.0were used. Growth studies and morphological comparisons by scanningelectron microscopy involved growing cells in tryptone-yeast extract-glucose(TYEG) broth and a minimal defined medium (MM4) (24), modifiedto contain Na/K phosphate buffer rather than phosphate-citratebuffer, and with the addition of 19 mM sodium carbonate. Escherichiacoli was maintained at 37°C (or 30°C when appropriate) on Luria-Bertaniplates and grown for plasmid isolations in Luria-Bertani broth.When appropriate, the following antibiotics were used at the indicatedconcentrations: erythromycin at 500 µg/ml for E. coli and 10 µg/mlfor S. mutans; tetracycline at 10 µg/ml for E. coli; and ampicillinat 100 µg/ml for E. coli.

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TABLE 1. Strains and plasmids used in this study

DNA methodology. The isolation of chromosomal and plasmid DNA, agarose gel electrophoresis, Southern hybridizations, DNA ligations, and transformationof E. coli were carried out as previously described (5), whilethe basic transformation procedures for S. mutans were as describedby Perry et al. (46). Sequencing was carried out manually usingSequenase (version 2.0; Amersham) with the modifications describedby Mytelka and Chamberlin (40) and automatically using fluorescentdye terminators provided by the University of Florida (Gainesville)DNA Sequencing Core Laboratory. Custom-made primers for manualsequencing or for PCR were synthesized by the University of Calgary,University Core DNA Services. PCRs were carried out using nativePfu polymerase (Stratagene) or the Expand Long Template PCR system(Boehringer Mannheim) according to manufacturers'instructions.

Isolation of S. mutans IS1A, G9IS1A, and BH97LC. S. mutans LT11 was transformed with pGh9:ISS1 essentially as described for Lactococcus lactis (38) with selection for plasmid-containingcolonies at 30°C on THYE-erythromycin plates. Plasmid-containingcultures were diluted 1:100 into fresh prewarmed medium withoutantibiotic and incubated for 3 h at 30°C to allow exponentialgrowth to resume. For transposition of pGh9:ISS1 into LT11, theculture was shifted to 37°C for 30 min and then to 42°C for 3h. Samples were diluted and spread on plates containing erythromycin(10 µg/ml) and incubated at 42°C for 1 to 2 days. To select forplasmid integrants, pH-sensitive mutants were isolated by picking~3,000 erythromycin-resistant colonies in duplicate onto THYEplates at pH 5.3 and pH 7.0. Approximately 90 colonies whose growthappeared to be impaired at pH 5.3 were picked in duplicate andplated onto THYE at pH 5.0 and pH 7.0. One colony (G9IS1A) thatshowed no growth at pH 5.0 wasselected.

Excision of the vector backbone was accomplished by growth without antibiotic at 30°C, plating dilutions onto solid medium.Individual colonies were then picked in duplicate and plated ontoselective (erythromycin [10 µg/ml] and non-selective medium andgrown overnight at 37°C. One colony out of 95 picked was erythromycinsensitive at 37°C, and the presence of ISS1 in the genome of thisstrain (IS1A) was confirmed by Southern hybridization (Fig. 1).Isolation of the regions flanking ISS1 were carried out by transformingIS1A with pISS1:r and selecting for erythromycin-resistant transformantsat 37°C. The presence of a pISS1:r intergrated via single-crossoverat the genomic copy of ISS1 was confirmed for five transformantsby Southern analysis. One was selected to attempt marker rescueand was named IS1A:r. Upstream and downstream regions were isolatedby rescue of the integrated copy of pISS1:r plus flanking DNAby digestion of IS1A:r DNA with either EcoRI or HindIII, ligationof the cut DNA, and transformation into E. coli XL1-Blue withselection for erythromycin resistance.

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FIG. 1. Construction and isolation of S. mutans G9IS1A and IS1A using pGh9:ISS1 and isolation of plasmids carrying DNA flanking the ISS1 element in IS1A. Thick lines and arrowheads represent genomic DNA, thin lines represent plasmid DNA, and small arrowheads represent ISS1 DNA. Abbreviations for restriction enzymes: E, EcoRI; H, HindIII.

To inactivate dltC in S. mutans LT11, plasmid pIS1A-MN was constructed by cloning the 1.35-kb MunI/NspV fragment from pIS1A/H:r,containing the 3' end of dltB, dltC, and the 5' end of dltD, intoEcoRI/ClaI-digested pBluescript KS. The dltC was disrupted bycloning an erythromycin resistance gene, isolated as a 1.8-kbBamHI fragment from pBS-Em, into the BglII site of pIS1A-MN togive pDLTC-Em (Fig. 2). Plasmid pDLTC-Em was linearized by digestionwith KpnI (single site in the vector) and used to transform LT11to erythromycin resistance. The presence of the interrupted dltCgene was confirmed for six transformants by Southern analysis,and one acid-sensitive clone was picked and named S. mutans BH97LC.

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FIG. 2. PCR products generated using S. mutans LT11 genomic DNA (lane 2), and S. mutans IS1A (lane 3) genomic DNAs as templates in reactions with primers ABC-UP and DLT-UP. Lane 1 shows the 1-kb ladder (Life Technologies) with sizes (in kilobases) shown on the left.

RNA isolation and RNA dot blotting. To isolate S. mutans RNA, log-phase cells were resuspended in 1 ml of TRIZOL reagent (Gibco-BRL) and disrupted by rapid shakingfor 24 s with glass beads using a Fast prep FP120 cell disruptor(Savant, Holbrook, N.Y.) according to the manufacturer's instructions.RNA preparations were treated with 20 U of RQ1 DNase (Promega)for 30 min at 37°C, extracted with TRIZOL and chloroform, andprecipitated with ethanol. The message for dltC and dltD was detectedby RNA dot blotting using the Genius nonradioactive nucleic acidlabeling and detection system (Roche Diagnostics, Laval, Quebec,Canada). A DNA probe was generated by amplifying a segment ofdltCD by PCR, using primer T7 and T3 with p7B/H-BgNs (Table 1)as the template. The probe was labeled directly during PCR usingdigoxigenin-dUTP following the manufacturer's (Roche) protocol.Equal amounts of total RNA extracted from parent strain LT11 andmutant BH97LC were applied to themembrane.

Characterization of BH97LC. The mutant was grown anaerobically in TYEG medium at pH 7.5, and log-phase cells were used to determined survival over thepH range pH 7.5 to 2.5 as previously described (50). Tests toexamine the ability of the mutant to initiate growth over thepH range 7.5 to 4.5 were carried out by inoculating (2%) the samemedium with an overnight culture of either the wild-type or mutantstrain. The ability of BH97LC to induce an ATR at sublethal pHvalues (pH 7.5 to 3.5) that would enhance survival over a 3-hperiod at pH 3.0 was determined by methods previously described(50).

D-Alanine incorporation assay. Incorporation of D-[¹⁴C]alanine into LTA by membrane and cytosolic (supernatant) fractions of the wild-type (LT11) and the mutant,BH97LC, was performed in reaction mixtures (50 µl) which contained30 mM bis-Tris (pH 6.5) 10 mM ATP, 10 mM MgCl₂, 1 mM dithiothreitol,and 0.11 mM D-[¹⁴C]alanine (43 mCi/mmol). The amount of incorporation was measuredby the method of Heaton and Neuhaus (28). For the preparationof membranes and supernatant fractions, cultures (500 ml) weregrown in TYEG medium and harvested at an optical density at 600nm of 1.6. The cells were washed in ice-cold water, suspendedin 10 ml of buffer containing 20% sucrose, 60 mM Tris-HCl (pH7.8), 2 mM MgCl₂, 0.25 g of lysozyme, and 1,000 U of mutanolysin(Sigma Chemical Co.); and incubated at 37°C for 2 h with gentleshaking. The resulting suspension was diluted 2.5 times with thesame buffer without sucrose and one tablet of the protease inhibitorcocktail (Boehringer Mannheim) was added. The disrupted cellswere further treated with a French press (three times at 15,000metric tons) and, subsequently, incubated with DNase and RNase.The supernatant fraction was centrifuged at 200,000 × g for 90min, and the membrane pellet was homogenized in a minimum amountof 30 mM Tris-HCl buffer (pH 7.8), 2 mM MgCl₂, and 10% glycerol.Membrane fragments were washed by two cycles of differential centrifugationat 9,000 and 200,000 × g and homogenized in the same buffer withaliquots frozen in liquid nitrogen and stored at $-$ 80°C. The 200,000× g supernatant was dialyzed against 30 mM Tris-HCl buffer (pH7.0) containing 2 mM MgCl₂ and 1 mM dithiothreitol and concentratedwith a Filtron centrifugal concentrator (10K; FiltronTechnologyCorp.).

Chemical analysis of LTA. LTA was isolated from early-stationary-phase cells following disruption in a Mickle disintegrator with Ballotini beads (60/40)and extraction by hot phenol-water. LTA was purified from theaqueous layer followed by hydrophobic chromatography on octyl-Sepharoseusing the centrifugation method of Koch et al. (35). The presenceof LTA in the final 50% 1-propanol fraction, following freeze-dryingand reconstitution in water, was confirmed in a precipitin reactionwith an anti-LTA antibody generated from L. rhamnosus ATCC 7469.The purified LTA was subjected to chloroform-methanol extraction(6) and analyzed essentially by the procedure of Perego etal. (45). One fraction was hydrolyzed in 2 M HCl at 100°C for2.5 h and analyzed for phosphorus (58), alanine (18), glucose(33), and glycerol (41) (analysis for glycerol following treatmentwith alkaline phosphatase). Alanine as the alanine ester and alanylglycerol were determined in the second fraction following mildalkaline treatment in 0.1 M NaOH at 37°C for 1 h. The chain lengthof LTA was calculated from the amounts (micromoles gram of drycells¹) of phosphorus and glucose using the following equation (45):phosphorus/0.5 glucose × 1.1.

Thin-section and scanning electron microscopy. Thin-section electron microscopy was performed essentially as previously described (26). Briefly, exponential-phase cellswere fixed overnight with 25% freshly purified glutaraldehyde,washed, and fixed for 1 h in 1% osmium tetroxide in SC-Mg buffer.Following additional washing and resuspension in 2% aqueous uranylacetate for postfixing, cell pellets were resuspended in an equalvolume of 3% low-melting-point agarose, and the resulting agarose-cellblocks were diced and dehydrated prior to thin sectioning. Silversections were mounted on uncoated hexagonal 400-mesh copper grids,stained first with saturated ethanolic uranyl acetate followedby 0.25% aqueous lead citrate in 0.1 M NaOH, and viewed and photographedat machine magnifications ranging from ×15,000 to ×100,000 ina Philips model 201 electron microscope at an acceleration voltageof 60KeV.

For scanning microscopy, cells were grown to exponential phase in TYE and in MM4 (24), the latter supplemented with 24 mMsodium bicarbonate, and then fixed overnight in cacodylate buffer(pH 7.4) containing 2.5% (wt/vol) glutaraldehyde at 4°C. Sampleswere then washed four times in 0.1 M cacodylate buffer, fixedto glass coverslips by a graded series of ethanol dehydrations,dried as previously described (10), and viewed with a HitachiS-2500 scanning electronmicroscope.

Proton permeability. The rate of proton uptake by intact cells of the wild-type and mutant strain was tested in a proton conductance assay usingenergy-depleted cells (20 mg [dry weight] ml¹) equilibrated at pH 6.0, 5.0, or 4.5 and receiving a pulse of10 mM HCl-140 mM KCl sufficient to drop the pH ~0.2 pH units (3,22). Washed cells were considered depleted of endogenous energyreserves when acid was no longer generated during anaerobic incubationat pH 7.0 in a pH-stat (22). The minimum pH of the suspensionimmediately after acid addition (pH) was reversed as protonsentered the cell and the extracellular pH increased. The pH recordingwas continued for approximately 10 min before butanol (6% finalconcentration) was added to permit complete equilibrium betweenthe cells and the external medium for the estimation of the finalequilibrated pH (pH). The results are expressed as the time(in minutes) required for the pH to reach a value (t_1/2) halfwaybetween pH and pH and are reported as the means ofat least three separatedeterminations.

Computer-aided analysis. Protein sequence analysis was carried out using the current version of the BLAST v2.0 homology search software (1) viathe World Wide Web interface of the National Center for BiotechnologyInformation (http://www.ncbi.nlm.nih.goc/BLAST). The sequenceof the genes shown in Fig. 2 has been submitted to the GenBankdatabase under accession number AF051356.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Isolation of acid-sensitive mutants. To isolate mutants of S. mutans LT11 unable to grow at pH 5.0, transposon mutagenesis with pGh9:ISS1 was used. Southern analysisof one erythromycin-resistant acid-sensitive colony (G9IS1A) indicatedthat a tandem transposition had occurred. From this strain, theplasmid backbone was excised leaving behind a single copy of theISS1 element (IS1A) (Fig. 1). Like G9IS1A, IS1A failed to growon THYE (pH 5.0) plates. The DNA flanking ISS1 was rescued bytransforming IS1A with pISS1:r to integrate a copy of the plasmidat this locus. This permitted recovery of genomic DNA fragmentscarrying the plasmid backbone plus additional flanking DNA (pIS1A/H:rand pIS1A/E:r [Fig. 1]). Sequence analysis of these flanking regionsfollowed by searches of the GenBank database showed that one endof ISS1 was inserted into a gene that had homology to dltB ofthe dlt operon (42), while the other end was inserted just upstreamof a gene whose product shows homology to proteins belonging tothe ATP-binding cassette (ABC) protein superfamily. Since theflanking regions were not genetically colinear, it was apparentthat a deletion had occurred during construction of G9IS1A andIS1A. PCR analysis, using primers to regions within the ABC anddltB sequences and using the LT11 genomic DNA as a template, revealeda 6.3-kb product representing the region deleted from IS1A (Fig.2, lane 2) and this was confirmed using IS1A genomic DNA as atemplate (Fig. 2, lane 3). This 6.3-kb PCR product and the ISS1flanking regions from pIS1A/E:r and pIS1/H:r were sequenced togive 11,202 bp of contiguous sequence comprised of nine completeopen reading frames (ORFs), eight of which were arranged in thesame orientation (Fig. 3).

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FIG. 3. Physical map and ORF characterization of 11,202 bp of the S. mutans LT11 genome based on DNA sequence analysis of pIS1A/E:r, pIS1A/H:r (plasmids rescued from strain IS1A carrying the flanking ends of the transposon and their junction sites), and the PCR product (hatched bar) produced using primers of the adjacent S. mutans DNA. The MunI/NspV fragment that was disrupted by insertion of an Em^r gene and used to construct pDLTC-Em is also shown. Hairpin structures represent putative transcriptional terminators. Genetic designations: ytqB, unknown; abcX, ABC transport protein; perM, permease; hlyX, hemolysin; pflC, pyruvate-formate lyase activase; dltABCD, genes of the dlt operon; ppx1, exopolyphosphatase. Abbreviations for restriction sites: B, BglII; E, EcoRI; H, HindIII; M, MunI; N, NspV; P, PstI, R, RcaI; S, SphI; X, XbaI.

As the size of the deletion precluded the possibility of assigning the acid phenotype of IS1A to any one gene, further workwas directed at the specific genes affected by the deletion. Anobvious starting point was the dlt operon, comprised of four genesencoding the proteins involved in the incorporation of D-alanineesters into LTA. Since these esters determine the polyanioniccharge of the cell surface, we addressed the role of this operonin determining the ATR of S. mutans LT11. The operon shared ahigh degree of similarity to previously reported sequences encodinggenes proven to be involved in D-alanyl-LTA synthesis in otherbacteria. For example, the deduced protein sequence of dltA (D-alanine-Dcpligase) from S. mutans LT11 shares 50% sequence identity withthe product of dltA of L. rhamnosus and 41% with the dltA productof B. subtilis (12, 45). As with the dlt operon of Lactobacilluscasei (27) and Streptococcus gordonii (10), dltA and dltBin S. mutans LT11 overlap as do dltC and dltD. In B. subtilis,the dlt operon also includes dltE, which encodes a protein belongingto a large family of oxidoreductases (45). We found no homologof dltE in the S. mutans LT11 sequence, but 61 bp downstream ofdltD is an ORF whose product has 76% sequence identity with aprotein (Cog) from S. gordonii, which is involved in intragenericcoaggregation (57). Further study of the BLAST search resultsrevealed that Cog was homologous to exopolyphosphatase encodedby the ppx1gene.

For inactivation of the dlt operon in S. mutans LT11, the gene (dltC) for the carrier protein, D-alanyl-Dcp, was disruptedsince the high specificity of the D-alanylation process appearsto be associated with this protein (42). We inactivated dltCby transforming S. mutans LT11 with linearized pDLTC-Em containingthe disrupted dltC gene (Fig. 3). Six erythromycin-resistant transformantswere shown by Southern analysis to have integrated the inactivedltC gene and all were acid-sensitive. One transformant, BH97LC,was subjected to furtherstudy.

Acid tolerance of BH97LC. From a variety of experiments, it was shown that BH97LC and IS1A were less acid tolerant than the wild-type strain LT11 (Table2). The data for these mutants showed that they were unable toinitiate growth below pH 6.5 compared to pH 5.0 for LT11 and hada higher killing pH (3.5) than LT11 (3.0). Further testing ofBH97LC demonstrated that the mutant exhibited a reduced capacityto induce an ATR. In the latter experiment, log-phase cells, grownat pH 7.5, were incubated for 2 h in the fresh medium at sublethalpH values (pH 6 to 4) to induce the ATR (24, 50) followedby a 3-h challenge at pH 3.0. This pH kills 100% of unadaptedcontrol cells maintained at pH 7.5 (50). As shown in Fig. 4,the response generated by BH97LC was significantly compromised,since the number of survivors at pH 3.0 was 3 to 4 orders of magnitudelower than that exhibited by LT11. Of particular interest forthe interpretation of this experiment was the fact that the terminalpH achieved during growth was only slightly higher (4.64) thanthat of the wild-type strain (4.50), suggesting that intracellularpH homeostasis could be maintained in the mutant once growth wasinitiated. In addition to the difference in ATR, the doublingtime of BH97LC was 2.8 times that observed for LT11, and the cellbiomass per mole of glucose was 0.66 times that of LT11 (Table2).

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TABLE 2. Growth and acid-tolerant characteristics of the wild-type strain S. mutans LT11 and acid-sensitive mutants

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FIG. 4. Effect of prior pH conditioning on the survival of the wild-type S. mutans LT11 and the mutant BH97LC in TYEG following a 3-h exposure to pH 3.0. Log-phase cells growing at pH 7.5 were transferred to fresh TYEG medium buffered at pH 6.0 to 3.5 and incubated at 37°C for 2 h prior to acidification to pH 3.0. The control cells (pH 7.5) were similarly treated. Error bars, standard deviations.

Incorporation of D-[¹⁴C]alanine into LTA. To confirm that the defect in the dltC gene had blocked D-alanine incorporation into LTA of BH97LC, permeabilized cells wereincubated with D-[¹⁴C]alanine and ATP according to the method of Ntamere et al. (43),and compared with permeabilized cells from parent LT11. Permeabilizedcells provide a test system for assaying the ligation of D-alanineto Dcp and its subsequent incorporation into mLTA. The incorporationof D-alanine in either toluene- or toluene-acetone-permeabilizedcells was 3% and <1% of that observed for the parent (data notshown). Thus, the insertion of the erm cassette in the dltC generesulted in the defective D-alanylation ofLTA.

By recombining the cytosolic (supernatant) fractions and membranes containing LTA from the parent and mutant in various combinations,it was determined that the defect was expressed in the cytosolicfraction. For example, the cytosolic fraction of BH97LC couldnot reconstitute the system with wild-type membranes (Table 3).To establish that BH97LC is deficient for Dcp, the cytosolic fractionfrom the mutant was reconstituted with recombinant Dcp from L.rhamnosus. Addition of 12.5 nM Dcp to this fraction reconstitutedthe maximum D-alanine incorporation observed with parent membranesand cytosolic fraction from the parent (Fig. 5). Thus, the dltCmutant, which is deficient for D-alanine incorporation, is deficientin Dcp.

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TABLE 3. Incorporation of D-[¹⁴C]alanine into LTA by in vitro combinations of membranes and cytosolic fractions from the wild-type strain S. mutans LT11 and the acid-sensitive mutant BH97LC

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FIG. 5. Reconstitution of the DltC-deficient cytosol fraction from BH97LC with Dcp. The D-alanine incorporation assay used was described in Materials and Methods, with the indicated amounts of membrane from either LT11 or BH97LC, cytosol (supernatant) fraction (3 µg of protein), and 12.5 nM Dcp.

Chemical analysis of wild-type and mutant LTA. In order to confirm the absence of D-alanylation of LTA in the mutant, the chemical compositions of the LTA from the wildtype and BH97LC were determined by extracting and purifying LTAfrom disrupted early stationary-phase cells under conditions maintainingD-alanine ester substitution of the LTA. The LTA from both thewild type and mutant was composed of poly(GroP) chains as indicatedby the equimolar ratio of glycerol and phosphorus (1.01 and 0.96,respectively), confirming values obtained earlier with purifiedLTA of S. mutans AHT (4). Furthermore, the LTA chain lengthsof the mutant and wild-type strains were essentially the same,e.g., 32 versus 36 glycerophosphate residues/chain, respectively.The molar ratio of D-alanine to LTA phosphorus for the wild type,LT11, was 0.67, slightly higher than that obtained with strainAHT (0.52) (4). The mutant, BH97LC, on the other hand, wasdevoid of D-alanine ester. Thus, chemical analysis confirms thatthe inactivation of dltC blocked D-alanine esterification of LTAand the formation of the poly(GroP) moiety of LTA wasunaltered.

Electron microscopy. Electron micrographs showed S. mutans LT11 to possess a fibrous extracellular matrix constituent that has also been reportedfor S. aureus (54). (Fig. 6A). There was no evidence of thismatrix material with the mutant BH97LC (Fig. 6B). Furthermore,unlike the wild type, cell wall thickness of the mutant variedwithin the same cell or diplococcal unit. One cell, or the endof a single cell, exhibited a thickness similar to LT11 cells,while polar caps of unequal thickness (Fig. 6B) were observedat the opposite ends of the diplococcal units (29). As seenin Fig. 7, comparisons of scanning electron micrographs of thewild-type and mutant cells grown on rich medium (TYEG) showedvirtually no difference in morphology, while a transfer to minimalmedium was correlated with a transition of the mutant cells fromdiplococcus to spheres which were not seen with the wild-typestrain, LT11.

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FIG. 6. Transmission electron micrographs of thin sections of the wild-type strain, S. mutans LT11, showing cell surface structures (A) (arrow) that are absent in the dltC-defective mutant, BH97LC (B) (arrow).

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FIG. 7. Scanning electron micrographs of log-phase cells of the wild-type strain, S. mutans LT11 (A and C), and in the dltC-defective mutant, BH97LC (B and D), grown in complex medium (TYEG) (A and B) and minimal defined medium (MM4) (C and D).

Proton permeability of the dltC mutant BH97LC. As the acid tolerance of oral streptococci has been shown to be related to the membrane permeability of protons (3, 22),we reasoned that the acid-sensitive mutant, BH97LC, may have adifferent permeability to protons than the wild-type strain, LT11.To test for differences in proton permeability, energy-depleted,log-phase cells of LT11 and BH97LC were equilibrated at pH 6.0,5.0, or 4.5 and then subjected to an acid pulse sufficient todrop the pH ~0.2 pH units (3). Proton uptake was determinedby extrapolation of the pH-versus-time curve from pH to pHachieved by the addition of butanol. Permeability was recordedas the t_1/2 value. As seen in Table 4, the lower t_1/2 valuesfor BH97LC at all pH values indicated the mutant was more permeableto protons than the wild-type strain. For example, at pH 4.5 themutant was almost twofold more permeable to protons that LT11.These results indicate that the defect in the dltC gene resultedin cells more permeable to the passive inflow of protons thanwild-type cells.

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TABLE 4. Proton uptake by deenergized cells of S. mutans LT11 (wild type) and the acid-sensitive mutant BH97LC as a function of the external pH^a

DltD expression in BH97LC. The insertion of the erm cassette into dltC may affect the synthesis of the complete polycistronic message. RNA dot blot analysisof the message for dltD indicated that the expression of thismessage was defective in BH97LC (Fig. 8). One of the functionsof DltD is to hydrolyze mischarged D-alanyl-ACP (13). Thus,hydrolysis of D-alanyl-ACP may be absent or greatly decreasedin the mutant membranes. In Fig. 9, the hydrolytic cleavage ofthe mischarged D-alanyl-ACP by the parent and mutant membranesis shown. At 5 min, 50% of the D-alanyl-ACP is cleaved by theparent membranes, whereas only 15% of this ligated-carrier proteinis hydrolyzed by the mutant membranes. In contrast, D-alanyl-Dcp,the normal carrier protein, is not hydrolyzed more than 5% byeither the mutant or wild-type membranes. Thus, the mutant describedin this paper would appear not only to be defective in the expressionof dltC, i.e., Dcp, but also for the expression of DltD. Thisdeficiency of DltD results from the upstream insertion of theresistance cassette.

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FIG. 8. Levels of message for dltC and dltD in the wild-type strain, S. mutans LT11, and the dltC-defective mutant, BH97LC, as detected by RNA dot blotting using a DNA probe of the dltC and dltD genes on p7B/K-BgNs as the template (Table 1).

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FIG. 9. Hydrolysis of D-alanyl-acyl carrier protein (ACP) and D-alanyl-Dcp by membranes from BH97LC and from LT11. Membranes from either the parent or mutant were incubated in a reaction mixture (250 µl) containing either 6.5 nmol of D-[¹⁴C]alanyl-ACP or D-[¹⁴C]alanyl-Dcp in 10 mM bis-Tris (pH 6.5) and 30 mM MgCl₂. Aliquots (50 µl) were removed from the mixtures at the indicated times, and the amount of D-[¹⁴C]alanyl-ACP or D-[¹⁴C]alanyl-Dcp remaining was measured by precipitation with 10% trichloroacetic acid according to the method of Heaton and Neuhaus (22).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The selection of the dlt operon for further study in relation to the acid-sensitive phenotype of mutant S. mutans BH97LC wasbased on the importance of D-alanyl-LTA in the growth and physiologyof gram-positive bacteria (2, 17, 34, 45, 56). To testfor a link between D-alanylation of LTA and acid sensitivity,we inactivated the dltC gene of the dlt operon in LT11, whichencodes the D-alanyl carrier protein, to create the mutant BH97LC.In addition to being unable to D-alanylate LTA, BH97LC was shownto be acid-sensitive, displaying a defective ATR and an increasedpermeability to protons compared to wild-typeLT11.

Inactivation of genes in the dlt operon in various bacteria shows an array of phenotypic changes. Insertional activation ofthe dltA-dltD genes in B. subtilis was without effect on LTA chainlength, cellular morphology, cell growth, and basic metabolismbut resulted in a greater susceptibility to methicillin and anincreased rate of autolysis (45, 55, 56). The latter ispostulated to occur by the increased binding of cationic autolysinsto the more negative, D-alanine deficient LTA. Similarly, recentstudies with Staphylococcus aureus and Staphylococcus xylosusdemonstrated that inactivation of the dlt operon resulted in enhancedsusceptibility of cells to positively charged antimicrobial peptides,such as defensin, protegrins, and similar compounds (47). Mutationof dltD in L. lactis resulted in slower growth than the wild-typestrain in addition to increased sensitivity to UV light (15).Inactivation of this gene in L. casei 102S resulted in an increasein cellular length and enhanced antimicrobial activity of thecationic detergents cetyltrimethylammonium bromide and chlorhexidine(13). In addition to the present study, two studies have examinedmutants defective in genes of the dlt operon in the oral streptococci.In one study, insertion of Tn916 upstream of the dlt operon inS. mutans UA130 resulted in cells deficient in glycogen-like storagematerial (49), while defects in dltA of S. gordonii DL1 resultedin loss of D-alanine esterification with the concomitant lossof intrageneric coaggregation and a 100-kDa surface protein associatedwith this aggregation (10).

In this study, the defect in the dltC gene resulted in a variety of alterations in growth characteristics in addition to theincreased acid sensitivity when compared to the wild-type strainLT11. For example, the doubling time was almost threefold longerthan that the wild-type, while the yield was 66% of that of LT11.Moreover, electron micrographs (Fig. 6) showed that the mutantwas devoid of the fibrous extracellular matrix observed with LT11,was typical of strains of S. mutans (39), and exhibited polarcaps of unequal thickness within the diplococcal unit. Comparisonsof the wild-type and mutant cells grown on TYEG showed virtuallyno difference in morphology, while a transfer to minimal mediumwas correlated with a transition of the mutant cells from rodsto spheres that was not seen with the wild-type strain LT11. Suchrod-to-sphere transition has been observed with S. mutans whenthe HCO₃/K⁺ ratio of the medium was increased (52). In the case of therod-to-sphere transition of the B. subtilis rodB1 mutant, thedegree of D-alanylation of wall teichoic acid decreased from 0.22to 0.10 at the restrictive temperature (48). Insertional inactivationof the dltA gene of S. gordonii DL1 resulted in a mutant (PK3241)with multiple septation sites, which also exhibited a smooth andunstructured surface with a thickened, cap-like cell wall similarto S. mutans BH97LC (10).

The relationship between the acid sensitivity of the mutant, BH97LC, and inactivation of LTA alanine esterification is currentlyunknown but may be related to alterations in normal pH homeostaticmechanisms. S. mutans responds to external acid over the shortterm by extruding protons from the cell via the membrane-associated,proton-translocating ATPase (H⁺ ATPase) (3, 22) and by acid end product efflux (11). Sustainedgrowth at low pH (5.5 to 5.0) results in increased H⁺ ATPase (22) and glycolytic activity (23). This is also supportedby a lowering of the pH optimum for sugar transport and glycolysis(22), as well as a shift in cellular regulation to increasedlactic acid formation (21) to support the efflux mechanism.Unlike the enteric bacteria (44), S. mutans does not maintaina constant intracellular pH (pHi) as the external pH falls butsupports a relatively consistent transmembrane pH gradient (~1.0U) that must be sustained by a carbon source (20). Thus, adaptationto growth at lower pH values permits the organism to maintaintransmembrane pH gradients at lower pH values (22).

These physiological characteristics can be used to explain the apparent paradoxical differences seen in Table 2 with respectto the acid sensitivity of BH97LC. The mutant was unable to initiategrowth below pH 6.5 and yet was able to lower the pH of an establishedgrowing culture to pH 4.64, just slightly higher than that ofthe wild-type strain. The carbon source, glucose, was essentiallydepleted during growth, and yet the yield was a third less thanthat of the wild-type. This observation suggests that the intracellularpH was maintained adequately by the H⁺ ATPase and lactate-efflux mechanisms (3), however, at a greatercost in ATP than that of the wild-type, resulting in a loss ofbiomass. This would suggest some alteration in the permeabilityof the mutant cells to protons that required cells to expend moreenergy to maintain the pH gradient. The inability to initiategrowth below pH 6.5 and the higher killing pH suggest that thecells are "leaky" to protons and can sustain a suitable intracellularpH only during active growth and glycolysis. The increased protonpermeability of deenergized cells of BH97LC compared to the wild-typestrain, particularly at pH 5.5 and 4.5, supports thisproposition.

Data presented here are consistent with our earlier findings (19), indicating a role for de novo membrane biogenesis inmaintaining an ATR. Specifically, we have shown that the signalrecognition particle-associated FFh ribonucleoprotein, which actsas a chaperone for the expedited insertion of newly synthesizedproteins into procaryotic membranes, is essential for a normalATR. In that work, we demonstrated reduced amounts of H⁺ ATPase in membranes of ffh mutants created by Tn917 insertions.It will be of great interest to determine if proteins associatedwith the dlt operon are also translocated by signal recognitionparticle-associatedmechanisms.

To our knowledge, the inactivation of dltC provides the first evidence linking increased proton permeability and the failureto induce a significant ATR, ensuring survival at a killing pH.This log-phase ATR requires protein synthesis and has been shownto involve the transient formation of proteins over a 2-h period(24). Thus, one might postulate that an alteration in the dltoperon resulting from the inactivation of dltC placed the cellsunder a condition of physiological stress, in which energy normallyrequired for protein synthesis during the ATR is diverted to pHhomeostasis. While one cannot exclude the possibility that thelower intracellular pH resulting from proton leakage may influencethe synthesis of specific proteins involved in the ATR, it ismore likely that the weak acid-induced adaptation is due to ageneral lack of biochemical or physiologicalfitness.

	ACKNOWLEDGMENTS

This research was supported by operating grants to I.R.H. (MT-3546) and D.G.C. (MT-15431) from the Medical Research Councilof Canada, by a grant to A.S.B. (DE-08007) from NIDCR, and bya Public Health Service grant (R01 GM51623) to F.C.N. from theNational Institute for General MedicalSciences.

We acknowledge the excellent technical assistance of Elke Greif and thank Paul Hazelton (University of Manitoba) for the electronmicrographs and Robert Chernecky (University of Toronto) for thescanning electronmicrographs.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Oral Biology, University of Manitoba, Winnipeg, Manitoba R3E 0W2, Canada.Phone: (204) 789-3615. Fax: (204) 789-3948. E-mail: ihamilt{at}umanitoba.ca.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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