Analysis of Functional Domains of the Enterococcus faecalis Pheromone-Induced Surface Protein Aggregation Substance

doi:10.1128/JB.183.19.5659-5667.2001

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Journal of Bacteriology, October 2001, p. 5659-5667, Vol. 183, No. 19
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.19.5659-5667.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Analysis of Functional Domains of the Enterococcus faecalis Pheromone-Induced Surface Protein Aggregation Substance

C. M. Waters and G. M. Dunny^*

Department of Microbiology, University of Minnesota Medical School, Minneapolis, Minnesota 55455

Received 18 December 2000/Accepted 12 June 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Pheromone-inducible aggregation substance (AS) proteins of Enterococcus faecalis are essential for high-efficiency conjugationof the sex pheromone plasmids and also serve as virulence factorsduring host infection. A number of different functions have beenattributed to AS in addition to bacterial cell aggregation, includingadhesion to host cells, adhesion to fibrin, increased cell surfacehydrophobicity, resistance to killing by polymorphonuclear leukocytesand macrophages, and increased vegetation size in an experimentalendocarditis model. Relatively little information is availableregarding the structure-activity relationship of AS. To identifyfunctional domains, a library of 23 nonpolar 31-amino-acid insertionswas constructed in Asc10, the AS encoded by the plasmid pCF10,using the transposons TnlacZ/in and TnphoA/in. Analysis of theseinsertions revealed a domain necessary for donor-recipient aggregationthat extends further into the amino terminus of the protein thanpreviously reported. In addition, insertions in the C terminusof the protein also reduced aggregation. As expected, the abilityto aggregate correlates with efficient plasmid transfer. The resultsalso indicated that an increase in cell surface hydrophobicityresulting from AS expression is not sufficient to mediate bacterialaggregation.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Enterococcus faecalis has become a growing health concern as a mediator of the spread of antibiotic resistance and a leadingagent of nosocomial infections (for review, see reference 10).The surface protein aggregation substance (AS) appears to playa role in both antibiotic resistance spread and in the pathogenesisof enterococcal infections. Expression of AS, which is encodedon the sex pheromone plasmids of E. faecalis, is induced by small7- to 8-amino-acid peptide pheromones (26). AS on the surfaceof the donor cell then binds its receptor, enterococcal bindingsubstance, on the recipient cell, mediating close cell contactthat leads to conjugative transfer of the plasmid. It is thoughtthat AS has no role in forming the DNA channel machinery, as efficientconjugation can occur if AS is expressed on either the donor orrecipient cells (26).

Over 20 different pheromone plasmids have been identified. Often, these pheromone plasmids express antibiotic resistance genesand other virulence factors, and many clinical isolates have multiplepheromone plasmids (36). The AS genes from the three most-studiedplasmids, Asa1 from pAD1, Asp1 from pPD1, and Asc10 from pCF10(encoded by the prgB gene), have been sequenced and show highidentity (see below). The gene encoding Asa373, the AS proteinof the pheromone plasmid pAM373, has also been sequenced but showslittle homology with the other known AS proteins and appears toaggregate through a different mechanism (21). Expression ofAS, which is normally tightly controlled in laboratory cultures,is induced in serum (13).

A number of functions of AS that may contribute to virulence have been identified. A major function of AS is host cell adhesion.Kreft et al. found that Asa1 increased adherence to cultured pigrenal tubular cells (13). Increased uptake mediated by Asc10into epithelial cells originating from the colon and duodenumbut not from the ileum has also been observed (25, 30). Alongthese lines, Asa1 increases invasion in an ex vivo model of thecolonic mucosa but does not increase translocation (11). Asc10has been found to increase adherence to and uptake by polymorphonuclearleukocytes, possibly by binding the integrin CR3 (35). In otherstudies, Asc10-expressing enterococci had higher intracellularsurvival rates in polymorphonuclear leukocytes (27). Likewise,adherence to and survival inside macrophages were increased withthe expression of Asa1 (33). In vivo examination of the roleof AS has centered on the rabbit experimental endocarditis model.Infection of a rabbit with a damaged heart valve leads to developmentof a mass of bacteria, platelets, and fibrin known as a vegetation(17). Two studies have found more severe vegetation formationinduced by AS-expressing enterococci (4, 31). Asc10 has alsobeen shown to increase adherence to fibrin and cell surface hydrophobicity(8).

Although much study has focused on the functions of AS, it is unclear how the structure of the protein mediates these functions.Like most gram-positive surface proteins, Asc10 has an N-terminalsignal sequence and C-terminal LPXTG cell wall anchor motif (seeFig. 1A). Analysis of the three sequenced genes encoding closelyrelated proteins reveals striking conservation of >90% identityin the majority of the protein, excluding a variable region of30 to 50% identity located between amino acids 266 and 559 inthe N terminus of AS (36). All three proteins also have conservedArg-Gly-Asp (RGD) motifs that have been implicated in bindingto integrins (13, 29, 33, 35). Secondary structural analysisyields little information with the exception of a predicted alpha-helixdomain from amino acids 200 to 280 (36). Isolation of AS yieldsboth a full-length version of the protein (137 kDa) and a specific,78-kDa, N-terminal cleavage product (9). Scanning electronmicroscopy of Asa1 on the cell surface suggests that the N terminusof the protein is more exposed than the C terminus (9). Finally,the only structural analysis of AS done to date found that anaggregation domain of Asa1 from amino acids 525 to 617 (of themature protein with the signal sequence removed) exists and thatthe C terminus plays no essential role in aggregation (20).

One dilemma with the use of conventional biochemical approaches to AS structure-function analysis is the high instabilityof purified protein. For this reason, we have taken a geneticapproach to probe the protein for functional domains using thetransposons TnlacZ/in and TnphoA/in (15, 16). In-frame insertionscan be identified by functional fusions to the 5' LacZ or PhoAreporter protein. Digestion of the insertion with BamHI removesmost of the transposon but leaves an in-frame 31-amino-acid insertion.These transposons have been successfully used to analyze the structure-functionrelationship of a number of membrane and cytosolic proteins (14,15, 19, 22, 23), but this is the first attempt to usethem in the analysis of a gram-positive surfaceprotein.

A library of 23 insertional mutants distributed throughout the length of the prgB gene has been constructed. The stabilityof the AS protein expressed by these mutants was examined, andmost proteins were found to be stable on the surface of E. faecalis.Phenotypic analysis of the insertion mutants in aggregation andconjugation revealed that both the N and C termini of the proteinplay significant roles in these processes. The ability of wild-typeand mutant Asc10 proteins to increase cell surface hydrophobicitywas also analyzed, and it was shown that increased hydrophobicityis not sufficient foraggregation.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains and culture conditions. E. faecalis was grown at 37 or 30°C as indicated with gentle shaking in Todd-Hewitt broth (Difco). For DNA isolation and manipulation,Escherichia coli was grown at 37°C with shaking in Luria-Bertani(LB) medium or brain heart infusion broth (Difco) for erythromycinselection. Agar plates contained 1.5% agar. The antibiotic concentrationsused for E. faecalis were erythromycin at 10 µg/ml, tetracyclineat 15 µg/ml, and rifampin at 200 µg/ml, while the concentrationsused for E. coli were erythromycin at 50 µg/ml (in brain heartinfusion broth) or 200 µg/ml (in LB) and chloramphenicol at 50µg/ml. All antibiotics were obtained fromSigma.

DNA manipulation. Plasmids were isolated with the Qiagen midi or mini kit as recommended by the manufacturer. Restriction enzymes were purchasedfrom Promega, Gibco BRL, and New England BioLabs. PCR was performedwith a Perkin-Elmer Gene Amp PCR system or a Eppendorf Mastercyclerusing either BioXact DNA polymerase (Bioline) or Vent polymerase(New England BioLabs). All sequencing and primer synthesis weredone by the Microchemical Facility of the University ofMinnesota.

Phage isolation, infection, and screening of transposon insertions. Preparation of $lambda$ TnlacZ/in and $lambda$ TnphoA/in was performed as previously described (1) using the E. coli suppressor strainCC245. Phage stocks were calculated at titers of 10⁷ phage/ml. Phage infection was performed as previously described(15) with some minor modifications. Cultures of E. coli strainCC160 containing the target plasmid were grown overnight to stationaryphase in $lambda$ broth (10 g of tryptone and 2.5 g of NaCl per litersupplemented with 0.2% maltose and 10 mM MgSO₄). One milliliterof the overnight culture was mixed with 1 ml of the phage stockand was incubated at 37°C for 10 min. Three milliliters of LBbroth was added, and the phage/bacteria were incubated at 30°Cwith gentle shaking for 6 h to overnight. The entire mixture wasplated (150- by 15-mm LB agar petri plates; Falcon) with erythromycinand chloramphenicol and was grown overnight. The colonies werecollected by washing the plates with distilled water. Plasmidswere isolated from these cells; electroporated into competentE. coli strain CC118; and plated on LB supplemented with erythromycin,chloramphenicol, 5% sucrose (to counterselect against right-endinsertions of the transposon), and 40 µg of 5-bromo-4-chloro- $beta$ -D-galactopyranoside(X-Gal) or 5-bromo-4-chloro-3-indolylphosphate (X-Phos) (Sigma)per ml. Blue transformants were screened by restriction digestionor colony PCR using a primer complementary to the nisin promoter(5'-CGGCTCTGATTAAATTCTGAAGTTTGTTAGATACAATGA-3') and to the insertionsequence (5'-CCTGGACGGAACCTTTCCCG-3'). Colony PCR was performedby mixing a sterile pipette tip touched to the side of a colonyinto the PCR mix. The bacterial cells were first lysed by a 10-min94°C incubation before the standard PCR was performed. The latterprimer in the insertion sequence was also used to sequence transposoninserts in prgB. The bulk of the transposon was removed with BamHI(Promega) digestion and religation with T4 DNA ligase (Gibco BRL).Relevant insertions in prgB were electroporated into E. faecalis,and transformants were screened by plasmid isolation (2) andrestrictiondigestion.

Construction of insertion mutants. Relevant plasmids are listed in Table 1. The initial target for insertion mutagenesis was the vector pMSP3602. This is aderivative of pINY1801 with the BamHI sites removed and was constructedin two steps. First, the blunt-ended KpnI-EcoRI fragment frompTRKH2 (the blunt end was generated using Klenow DNA polymerase[Promega] with the manufacturer's instructions) containing theerythromycin gene was inserted into the BanII site of pINY1801to generate pMSP3601. The BamHI fragment from pMSP3601 was removedwith BamHI digestion, and the overhangs of the fragment and vectorbackbone were filled with Klenow polymerase. The blunt-ended fragmentwas then religated into the pMSP3601 backbone to create pMSP3602.The TnlacZ/in insertions $Omega$ 1077, $Omega$ 1638, $Omega$ 2049, $Omega$ 2064, $Omega$ 2085, $Omega$ 2421, $Omega$ 2601, $Omega$ 2979, $Omega$ 3102, $Omega$ 3414, and $Omega$ s3599 (Fig. 1) were generatedin pMSP3602. $Omega$ s3599 is an out-of-frame insertion at the very Cterminus of the gene, resulting in production of most of the geneproduct without a cell wall anchor. The amino acid insertion sequencegenerated by the in-frame insertion sequence is 5'-XDSYTQVASWTEPFPFSIQGDPRSDQETXXX-3',where X depends on the duplicated target sequence. Due to a lackof prgB expression in pMSP3602, these insertions were moved intopMSP7517 by isolating the prgB BsrGI-BlpI fragment containingthe insertion from pMSP3602 and by ligating it into pMSP7517,replacing the corresponding wild-type prgB sequence. pMSP7517was also used as a target for insertional mutagenesis generating $Omega$ r2760 and $Omega$ r3183. These insertions are in frame but are in thereverse orientation, generating the amino acid insertion sequence5'-XXXCLLIRSWIPLDGKRERFRPGRYLCIRVS/R-3', where X depends on theduplicated target sequence. Out-of-frame and reverse insertionswere frequently observed, as the transcription machinery of E.coli was likely recognizing artifactual promoters in the AT-richE. faecalis DNA. In an attempt to decrease the target size ofthe gene, pMSP7517 $Delta$ MscI was constructed by removing the MscI fragmentfrom pMSP7517. Two TnphoA/in insertions, $Omega$ 96 and $Omega$ 258, were generatedin this construct. These insertions were restored to the contextof full-length prgB by reinserting the prgB MscI fragment intothe MscI restriction site. Note that the insertions left afterremoval of the BamHI fragments are identical for both $lambda$ TnlacZ/inand $lambda$ TnphoA/in.

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TABLE 1. Strains and plasmids used in this study

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FIG. 1. (A) The positions of insertion mutations in prgB are shown on a linear map of the gene. Each mutation consists of an in-frame 31-amino-acid insertion. The insertions at r2760 and r3183 are in frame but in the reverse orientation, while the insertion at s3599 is out of frame and produces a stop codon. Structural map: SS, signal sequence; helix, predicted N-terminal helix domain; variable, unconserved AS region; essential, aggregation domain identified by Muscholl-Silberhorn; and cleavage, site of cleavage that produces the characteristic N-terminal 78-kDa fragment. (B) The mutant Asc10 proteins were expressed using the nisin-inducible Asc10 expression vector pMSP7517.

A lack of N-terminal insertions in prgB led to the hypothesis that these fusions were lethal for E. coli, possibly througha protein hybrid jamming mechanism (32). To overcome this problem,a signal sequence-deficient clone of prgB was generated and wasinserted into the vector pGEX-4T to create pMSP3604. pMSP3604was constructed in two steps. A PCR product from the BsrGI (5'-AGAGATCTACTGATAATGTACAAGC-3',with a BglII site)-to-BtrI (5'-TAGGCTTAAGAAGCAGTCACGTCTTTCGC-3',with an EcoRI site) sites of prgB in pMSP7517 was generated withBioXact and was cloned into the pGEM-T Easy (Promega) vector togenerate pMSP3603.1. No erroneous mutations were found in thePCR product as determined by sequencing. The prgB fragment wasremoved by BglII-EcoRI digestion and was ligated into the BamHI-EcoRIsites of pGEX-4T, creating pMSP3604. The insertions $Omega$ 324, $Omega$ 438, $Omega$ 468, $Omega$ 1074, $Omega$ 1299, $Omega$ 1317, $Omega$ 1419, and $Omega$ 1551 were generated inpMSP3604. These insertions were moved back into pMSP7517 in thecontext of wild-type prgB using two approaches. Initially, theBsrGI-BtrI fragment containing the insertion was isolated andwas exchanged with pMSP7517. However, problems with the BtrI restrictionenzyme forced some of the insertions to be moved by isolatingthe BsrGI-PshAI fragment containing the insertion from pMSP3604and exchanging it with the same fragment ofpMSP7517.

Nisin induction, surface extraction, and Western blotting. For nisin induction, cultures inoculated 1% from an overnight culture were grown for 3 h in Todd-Hewitt broth plus the appropriateantibiotics with gentle shaking. Nisin was added to a final concentrationof 25 ng/ml (a stock solution of 10 mg of nisin/ml was made froma 2.5% nisin preparation [Sigma] in distilled water [effectivenisin concentration was 250 µg/ml]), and the cultures were incubatedfor an additional 1.5 h. To overcome the differences in growthrate, the cultures grown for the stability difference seen at30°C were induced overnight with 25 ng of nisin/ml. A lysozymesurface extract of each induced mutant culture was performed aspreviously described (7). The lysozyme extraction buffer wasslightly modified to include 12.5 mM EDTA and 25 mg of lysozyme/mlfor the extraction of the four cultures grown at 30 or 37°C tomeasure differences in protein stability. The protein concentrationof each sample was determined using the bicinchoninic acid ProteinAssay Kit (Pierce). An equivalent amount of each sample was electrophoresedon a sodium dodecyl sulfate-7.5% polyacrylamide gel electrophoresisgel and was transferred to a BA 85 nitrocellulose membrane (Schleicher& Schuell). Western blot analysis was performed with an antibodyconstructed against an N-terminal domain of Asc10 (18) at adilution of 1/2,500. Detection was performed with the enhancedchemiluminescence protocol(Pierce).

Quantification of aggregation using flow cytometry and spectrophotometry. Aggregation was quantified by two methods. Nisin-induced cultures were directly diluted 1/5 in phosphate-buffered saline-0.1%Tween 20 and were analyzed on a Becton Dickinson FACScan, andthe data were analyzed using CellQuest Version 3.3 software (BectonDickinson). Identically placed quadrants were used to analyzethe percentage of each sample in each quadrant. One milliliterof nisin-induced cultures was also poured into plastic cuvettesand was left stationary for 1 h. The optical density at 600 nm(OD₆₀₀) of each sample was read on a Beckman DU-70Spectrophotometer.

Plasmid transfer. The insertional mutants were induced with nisin as previously described with the exception that no antibiotic was added tothe medium. The donor strain, OG1SSp(pCF175), an Asc10 pCF10 derivative, was induced in the same manner except that25 ng of cCF10/ml was added instead of nisin. The recipient strainsexpressed either wild-type Asc10 or one of the insertion mutants,as AS can increase plasmid transfer when expressed on either thedonor or recipient cell. The induced donor and recipient cultureswere mixed at a ratio of 1:10 respectively and were incubatedat 37°C for 30 min. Transconjugants were enumerated by serialdilution on Todd-Hewitt broth with rifampin andtetracycline.

Hydrophobicity assay. Cell surface hydrophobicity was measured using a hexadecane extraction of induced cultures as previously described (28).Hydrophobicity is expressed as the percentage of cells that areextracted to the hexadecane as measured byOD.

Statistical analysis. Statistical significance was calculated by determining confidence intervals for the differences of two population means whenpopulation variances are known (12).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction of PrgB insertion mutants. To scan Asc10 for potential functional domains, the transposons TnlacZ/in and TnphoA/in were used to generate in-frame, nonpolar31-amino-acid insertion mutations throughout prgB (15, 16).Previous work with the well-defined LacI repressor protein usingthese transposons identified the important functional motifs,validating their use in structure-function analysis of less-well-definedproteins (22). Briefly, prgB, carried on a shuttle plasmid,was targeted by TnlacZ/in or TnphoA/in in E. coli strain CC160.Relevant insertions were isolated and sequenced. The bulk of thetransposon was then removed from prgB by BamHI restriction digestionand religation, leaving a 31-amino-acid in-frame insertion. The31-amino-acid insertion consists of 84 bp provided by the transposonand 9 bp derived from the duplicated target sequence. The prgBinsertions were electroporated into E. faecalis and were analyzedfor surface expression, loss of function of aggregation and ofconjugation, and increase in cell surface hydrophobicity. Thedesignation of the insertion mutations generated in this studyindicates the nucleotide residue of prgB that immediately precedesthe insertion junction (Table 1). A number of different plasmidswere used to construct the insertion mutants (see Materials andMethods for rationale), but all of the functional analysis wasperformed with the insertions in the prgB gene of the nisin-inducibleconstruct pMSP7517, allowing for controlled expression of themutations.

Analysis of surface localization of Asc10 mutants. The stability of the mutant proteins was addressed by analyzing their surface expression in E. faecalis. Surface expressionof the Asc10 insertion mutations in E. faecalis was analyzed bygenerating cell wall extracts of each mutant (7). An equivalentamount of total protein (measured by a bicinchoninic acid proteinassay [Pierce Chemical] and silver staining) was electrophoresedon a Sodium dodecyl sulfate-polyacrylamide gel electrophoresisgel and was Western blotted with a polyclonal antibody generatedagainst the first 333 amino acids of Asc10 (18) (Fig. 2). Whenisolated from the cell wall, wild-type AS becomes very unstableand usually forms a laddering pattern on a Western blot. Mostof the surface protein extracts from the insertion mutants reactedwell in a Western blot, indicating normal cell wall localization.Only three mutants, $Omega$ 324, $Omega$ 2049, and $Omega$ 2064, had reduced levelsof reactive protein. One mutant, $Omega$ 2085, had no reactive proteinon the cell surface and was removed from the functional analysis.Surprisingly, $Omega$ s3599, which has no cell wall anchor, also hadreactive protein on the cell surface. Likely, anchorless Asc10released from the cell immediately binds the AS receptor, enterococcalbinding substance, on the cell surface. A Western blot of $Omega$ s3599expressed in the enterococcal strain INY3000 (negative for enterococcalbinding substance) (34) had no reactive protein on the surfaceof the cell (data not shown). The mutant proteins also have differentladdering patterns on the Western blot, suggesting differencesin protein stability on the surface of the cell or during theextraction procedure. When different preparations of the samemutant protein were examined on different blots, they exhibitedvariable laddering patterns, making it difficult to draw conclusionsabout the mutant stability from the laddering patterns.

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FIG. 2. Western blot analysis of surface extracts from the Asc10 insertion mutants. The Western blot utilized a polyclonal antibody generated against the N terminus of Asc10. An equivalent amount of protein was added to each lane. The laddering pattern is typical of AS protein preparations, as they have high instability. Migration of molecular mass standard marker proteins is shown at the left of the blot, and the 137-kDa full-length Asc10 and 78-kDa fragment are indicated by arrows. 7517, Asc10⁺; 3535, vector control.

Identification of two domains that mediate aggregation. Aggregation of the insertion mutants was quantified by two methods. Figure 3A shows representative data from five mutants.First, the forward scatter and side scatter profiles of inducedcultures were determined on a flow cytometer. Larger particleshave larger forward scatter and side scatter profiles. Populationswere separated into four quadrants (Fig. 3A, bottom). The vectorcontrol (3535) had very few events located in the upper rightquadrant (0.03%), while a much larger percentage of the wild-typeAsc10 nisin-induced (7517) population was located in the upperright quadrant (4.65%) (Fig. 3A and B). The profile of each mutantswas determined two to three times (Fig. 3B). Many mutations throughoutthe gene resulted in complete inhibition of aggregation, whileothers maintained wild-type aggregation levels. Some mutants, $Omega$ 1077, $Omega$ r2760, and $Omega$ r3183, had intermediate levels of aggregation. $Omega$ 1317 and $Omega$ 1419 had very low but statistically significant levelsof aggregation. Interestingly, $Omega$ 1299, $Omega$ 2064, and $Omega$ 3414 had statisticallysignificant, increased levels of aggregation relative to wild-typeAsc10. As expected, $Omega$ s3599 was unable to aggregate.

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FIG. 3. Aggregation of the mutants was measured by spectrophotometry and flow cytometry. Representative data for Asc10⁺ (7517), the vector control (3535), a functional mutant (1299), intermediate mutant (r2760), and a nonaggregating mutant (3102) are shown. UR, upper right. (A). The aggregation of the mutants was measured by flow cytometry as a percentage of the induced populations in the (UR) quadrant (B). The OD₆₀₀ of induced cultures after 1 h of settling was also determined (C). A decrease in OD₆₀₀ indicates aggregation. #, P < 0.05 from 7517; @, P < 0.1 from 7517; *, P < 0.05 from 3535; $, P < 0.1 from 3535.

Aggregation was also quantified by determination of the OD₆₀₀ of induced cultures after 1 h of settling (Fig. 3A, top, andC). For these data, increased aggregation is indicated by a decreasedOD. Data obtained in this manner generally agreed with the resultsgenerated on the flow cytometer. In this method, no significantdifferences could be distinguished between cells expressing wild-typeAsc10 and cells expressing mutant proteins that were functionalaggregators. Likewise, no statistical difference was found betweenvector control 3535 and the nonaggregators $Omega$ 1317 and $Omega$ 1419. However,mutants displaying an intermediate level of aggregation when measuredon the flow cytometer ( $Omega$ 1074, $Omega$ 1077, $Omega$ r2760, and $Omega$ r3183) werealso intermediate when measured by the spectrophotometer. Comparisonof the two methods suggests that flow cytometry is more sensitivein quantifying small differences in aggregationlevels.

The data measured by these two methods indicated a distinct aggregation domain expressed in the gene from nucleotide residues1317 to 1638 (corresponding to amino acids 439 to 663 of the Asc10protein). Also, many insertions in the C terminus ( $Omega$ 2421, $Omega$ r2760, $Omega$ 3102, and $Omega$ r3183) had reduced or abolished aggregation, indicatingregions in the C terminus that are involved in aggregation. However,two C-terminal functional aggregators ( $Omega$ 2601 and $Omega$ 2979) were interspersedamong the nonaggregators, suggesting that the entire region doesnot participate inaggregation.

Temperature-sensitive stability of Asc10 from $Omega$ 2049 and $Omega$ 2421. Growth of $Omega$ 2049 and $Omega$ 2421 at 30°C resulted in increased aggregation to near-wild-type levels (Fig. 4A). Analysis of surfaceextracts of these strains by Western blotting revealed that muchhigher levels of Asc10 were isolated from cells grown at 30°C.Note that increased exposure times would show reactive proteinin the 37°C extract of 2421, confirming the presence of reactiveprotein seen in Fig. 2. Interestingly, more wild-type Asc10 canbe seen from cultures grown at 30°C as well (Fig. 4B). These datasuggest that the failure of $Omega$ 2049 and $Omega$ 2421 to aggregate at 37°Cwas likely due to instability of the mutant proteins rather thanto disruption of an aggregation functional domain. The mechanismof this increased stability at 30°C is unknown. Growth at 30°Cdid not affect the aggregation phenotype of any of the other insertionmutants.

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FIG. 4. Insertion mutants 2049 and 2421 have near-wild-type aggregation levels when grown at 30°C as indicated by spectrophotometry (A). Western blot analysis of surface extracts indicated much more reactive protein on these cells when they were grown at 30°C (B). Migration of molecular mass standard marker proteins is shown to the left of the blot, and the 137-kDa full-length and 78-kDa Asc10 fragments are indicated by arrows.

Plasmid transfer of insertion mutants correlates with aggregation. To determine the plasmid transfer capability of the insertion mutants, nisin-induced mutant cultures were used as recipientsand were mixed with an E. faecalis OG1SSp(pCF175) donor strain.pCF175 is a pCF10 derivative that has a Tn917 insertion in theprgB gene, rendering it incapable of aggregation or efficientconjugation. Thus, aggregation could only be mediated by the recipientAsc10 mutants, as expression of AS can lead to increased conjugationwhen expressed on either the donor or recipient cell of the matingpair (26). Plasmid transfer is expressed as the number of transconjugantcells/donor cell. As expected, induced 7517 gave high transferlevels at 3.5 × 10², while the vector control transferred at 6.5 × 10⁴. Various transfer levels were observed for the mutants (Fig.5A), and as expected, transfer levels correlated with aggregationability (Fig. 5B). Interestingly, the three mutants that had significantlyhigher aggregation levels as measured by flow cytometry, $Omega$ 1299, $Omega$ 2064, and $Omega$ 3414, did not have statistically significantly highertransfer levels.

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FIG. 5. The plasmid transfer levels of each mutant were determined and were expressed as transconjugants/donor (tc/donor) (A). Plasmid transfer levels are compared with the ability to aggregate (B). UR, upper right.

Hydrophobicity. Cell surface hydrophobicity of the insertion mutants was measured by determining the percentage of cells that could be extractedfrom aqueous solution into hexadecane (Fig. 6A). A number of mutantsmaintained high levels of cell surface hydrophobicity, with somemutants having an even higher percentage of cell surface hydrophobicitythan wild-type Asc10. Likewise, many mutants showed low levelsof surface hydrophobicity comparable to those of non-Asc10-expressingstrains. The amino acid sequences generated by both the forwardand reverse insertions are relatively hydrophilic, with a percentageof polar amino acids at 63 and 50%, respectively. However, theactual amino acids of the insertion seemed to have little effecton the overall hydrophobicity of the mutants. The hydrophilicity,surface probability, and antigenicity indices were calculatedfor the amino acid sequence of Asc10 using the program PEPTIDESTRUCTURE(Wisconsin Package Version 10.1; Genetic Computer Group [GCG],Madison, Wis.). The values for a window of 10 amino acids adjacentto the insertion mutations were not predictive of the effect oncell surface hydrophobicity (data not shown).

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FIG. 6. Cell surface hydrophobicity of each mutant as a percentage of cells that were extracted with hexadecane (A). Comparison of hydrophobicity with aggregation for each mutant can be seen in the scatter plot (B). UR, upper right.

The effect of cell surface hydrophobicity on aggregation was examined by plotting aggregation ability on the x axis versusthe percent hydrophobicity on the y axis (Fig. 6B). No strongcorrelation between cell surface hydrophobicity and aggregationlevels wasobserved.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The functional analysis of the 23 prgB insertion mutants generated in this study led to four important conclusions: (i) thedomain that mediates bacterial aggregation extends into the variableregion of Asc10, farther into the amino terminus than previouslyreported (13), (ii) the C terminus of the protein does contributeto aggregation, (iii) efficient conjugation directly correlateswith functional aggregation, and (iv) increased cell surface hydrophobicitycaused by Asc10 is not sufficient to mediateaggregation.

The transposons TnlacZ/in and TnphoA/in have been successfully used to analyze the structure-function relationship of a numberof gram-negative membrane and cytosolic proteins (14, 15,22, 23) and even a mouse mammary tumor virus superantigen(19), but to our knowledge, this study is the first attemptto use these transposons for mutagenesis of a protein from a gram-positiveorganism. Although we had problems with E. coli transcriptionmachinery recognizing artifactual promoters and inefficient exportof the fusion proteins, 23 nonpolar, in-frame 31-amino-acid insertionswere generated that were spaced throughout the prgB gene. Theinsertion mutants have good coverage of the protein, with thelargest gap found from nucleotide residues 468 to 1074. This regionwas resistant to transposition, as multiple mutagenesis attemptsyielded no insertions. Interestingly, previous Tn5 mutagenesisstudies that targeted pCF10 DNA also had a large gap in the prgBgene that corresponds to the same transposition-resistant regionidentified in this study (26).

Western blotting of the surface extracts of induced mutant cultures revealed that most proteins were expressed on the surfaceof the cell. Full-length protein was difficult to observe in somemutants, but this result is not unexpected, as purified proteinis very unstable. Three mutants, $Omega$ 324, $Omega$ 2049, and $Omega$ 2064, had reducedexpression of Asc10 at 37°C, while $Omega$ 2085 showed no reactive protein.Consequently, $Omega$ 2085 was removed from the functional analysis.Interestingly, the insertion mutants $Omega$ 2049 and $Omega$ 2421 were foundto aggregate to near-wild-type levels when grown at 30°C, suggestingthat their lack of aggregation at 37°C is due to protein instability.The increased stability of these proteins at 30°C may be due toalterations in folding conformations or differences in activityof an enterococcal cell surfaceprotease.

Insertions in two major regions of the protein inhibited or abolished aggregation. Insertions in the N terminus inhibitedaggregation in agreement with Muscholl-Silberhorn's previous identificationof an aggregation functional domain for Asa1 (20). The insertionsgenerated in this study identify an aggregation functional domainin the gene from nucleotide residues 1317 to 1638, but it is notclear how far the functional domain extends beyond residue 1638.However, as $Omega$ 2049 aggregates at 30°C, the aggregation domain doesnot extend this far into the gene. The aggregation domain identifiedin Asa1 extends from base numbers 1704 to 1980. Combining thetwo identified regions would indicate an aggregation domain from1317 to 1980 (Fig. 7). Also, a comparison of the two results indicatesthat the aggregation functional domain for Asc10 extends fartherinto the amino terminus of the protein than previously reportedfor Asa1. Interestingly, the domain identified in this study extendsinto the variable region, suggesting that it may play a role inaggregation. This result is supported by the observation thatan Asa1-AspI variable region chimera fails to aggregate (20).Most of the insertions in the extreme N terminus of the protein,residues 258 to 1299, had no effect on aggregation levels withthe exception of $Omega$ 96 and $Omega$ 324. Mutation $Omega$ 96 was in the signalsequence of the protein and likely disrupted correct migrationthrough the cell membrane, while $Omega$ 324 had very low protein levelson the cell surface, suggesting decreased stability of the protein.

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FIG. 7. Functional domains identified in this study that disrupted aggregation (top) and hydrophobicity (bottom). All proteins generated from these insertions were expressed on the cell surface. The two mutants with increased stability at 30°C are indicated (*). Amino acids preceding the insertions indicate the mutants (nucleotide residues are given in parentheses). The Extended Agg domain was identified by the mutations in this paper and by the previously identified aggregation functional domain (21). Note that the N-terminal aggregation domain extends into the variable region. C-terminal insertions that disrupt aggregation are hypothesized to play a structural role. Many mutants that are unable to aggregate still increase cell surface hydrophobicity.

Surprisingly, some C-terminal insertions had reduced or abolished aggregation. Specifically, the protein produced by insertions $Omega$ r2760, $Omega$ 3102, and $Omega$ r3183 were expressed well on the cell surface.These mutants also reacted with an anti-Asc10 monoclonal antibodyas measured by fluorescence-activated cell sorter analysis (datanot shown), further indicating reactive protein on the cell surface.Strikingly, the insertion at $Omega$ 3102 was completely deficient inaggregation. In contrast, Muscholl-Silberhorn (20) concludedthat the C terminus of Asa1 is not essential in aggregation basedon two observations: (i) a C-terminal deletion construct maintainsaggregation, although at a third of wild-type levels, and (ii)an N-terminal fragment of the protein attached to a solid surfacecan mediate cell attachment. Based on (i) the data reported inthis paper, (ii) the preceding observations with Asa1, and (iii)the fact that the N terminus is more surface exposed (9), itis likely that the C terminus plays a structural role in aggregation.Specifically, the regions identified by the insertions $Omega$ r2760, $Omega$ 3102, and $Omega$ r3183 serve to place the N-terminal functional domainin the correct conformation to mediate aggregation. This hypothesiscould account for the decreased aggregation seen in the C-terminaldeletion of Asa1. Moreover, the structural function of this C-terminaldomain may not be necessary when the protein is attached to asolid surface, as observed by Muscholl-Silberhorn (20). Notethat the fully functional insertion $Omega$ 2979 intersects this structuralregion, indicating that some sites are permissive. It should benoted that the use of these transposons in the analysis of structure-functionrelationships has been validated by previous work with the LacIrepressor (22). In this study, all 18 31-codon insertions generatedby random transposition of TnlacZ/in yielded the predicted phenotypesbased on previous structural analysis of theprotein.

As expected, the ability to aggregate positively correlated with plasmid transfer levels, further supporting the notion thatthe only role of AS in conjugation is to initiate close contactbetween the members of the donor-recipient pair. Interestingly,the mutants that had statistically significant higher levels ofaggregation as measured by flow cytometry did not have higherlevels of plasmid transfer, suggesting that AS has evolved aggregationlevels that maximize plasmidtransfer.

The increased cell surface hydrophobicity elicited by Asc10 expression was also measured for each mutant. Various levels ofhydrophobicity could be seen for the insertion mutants, but noone distinct domain necessary for increasing hydrophobicity wasdetected. Comparison of the hydrophobicity and aggregation levelsreveals that increased cell surface hydrophobicity is not sufficientfor aggregation. Specifically, $Omega$ 1551 is unable to aggregate butinduces very high levels of cell surface hydrophobicity. Likewise,mutants that are intermediate aggregators have hydrophobicitylevels equivalent to those of strong aggregators. Thus, AS mediatesaggregation through a specific interaction, as opposed to a generalizedalteration of cell surface hydrophobicity. It should be notedthat no mutants that were completely deficient in increased cellsurface hydrophobicity were able to aggregate, possibly indicatingthat hydrophobicity may be necessary but not sufficient foraggregation.

This study reports the construction of a library of 23 31-amino-acid insertions in Asc10, the AS of pCF10. By using Westernblotting of surface extracts, it was shown that most of the insertionmutants were expressed on the surface of E. faecalis. Analysisof aggregation identified both N- and C-terminal domains importantin aggregation and showed that the variable region may play arole in aggregation. Moreover, an increase in cell surface hydrophobicityis not sufficient for aggregation. This insertion library willbe further analyzed for functional domains of Asc10 involved inthe pathogenesis of E. faecalisinfections.

	ACKNOWLEDGMENTS

We thank Colin Manoil for supplying the transposons used in this study and for helpful advice. We thank Pat Cleary for readingthe manuscript and Pat Schlievert, Helmut Hirt, and John McCormickfor providing antibodies, other reagents, and helpfuldiscussion.

This work was supported by NIH grants GM-49530 and HL-51987. C.M.W. was supported by NIH training grant 5 T32 AI07421-5.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, University of Minnesota Medical School, 1420 Delaware St.SE, Minneapolis, MN 55455. Phone: (612) 625-9930. Fax: (612) 626-0623.E-mail: gary-d{at}biosci.cbs.umn.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl. 1990. Current protocols in molecular biology. John Wiley & Sons, Inc., New York, N.Y.

2. Bae, T., S. Clerc-Bardin, and G. M. Dunny. 2000. Analysis of expression of prgX, a key negative regulator of the transfer of the Enterococcus faecalis pheromone-inducible plasmid pCF10. J. Mol. Biol. 297:861-875[CrossRef][Medline].

3. Bryan, E. M., T. Bae, H. Kleerebezem, and G. M. Dunny. 2000. Improved vectors for nisin-controlled expression in gram-positive bacteria. Plasmid 44:183-190[CrossRef][Medline].

4. Chow, J. W., L. A. Thal, M. B. Perri, J. A. Vazquez, S. M. Donabedian, and D. B. Clewell. 1993. Plasmid-associated hemolysin and aggregation substance production contribute to virulence in experimental enterococcal endocarditis. Antimicrob. Agents Chemother. 37:2474-2477[Abstract/Free Full Text].

5. Christie, P. J., and G. M. Dunny. 1986. Identification of regions of the Streptococcus faecalis plasmid pCF-10 that encode antibiotic resistance and pheromone response functions. Plasmid 15:230-241[CrossRef][Medline].

6. Dunny, G. M., B. L. Brown, and D. B. Clewell. 1978. Induced cell aggregation and mating in Streptococcus faecalis: evidence for a bacterial sex pheromone. Proc. Natl. Acad. Sci. USA 75:3479-3483[Abstract/Free Full Text].

7. Galli, D., F. Lottspeich, and R. Wirth. 1990. Sequence analysis of Enterococcus faecalis aggregation substance encoded by the sex pheromone plasmid pAD1. Mol. Microbiol. 4:895-904[CrossRef][Medline].

8. Hirt, H., S. L. Erlandsen, and G. M. Dunny. 2000. Heterologous inducible expression of Enterococcus faecalis pCF10 aggregation substance Asc10 in Lactococcus lactis and Streptococcus gordonii contributes to cell hydrophobicity and adhesion to fibrin. J. Bacteriol. 182:2299-2306[Abstract/Free Full Text].

9. Hirt, H., G. Wanner, D. Galli, and R. Wirth. 1993. Biochemical, immunological and ultrastructural characterization of aggregation substances encoded by Enterococcus faecalis sex-pheromone plasmids. Eur. J. Biochem. 211:711-716[Medline].

10. Huycke, M. M., D. F. Sahm, and M. S. Gilmore. 1998. Multiple-drug resistant enterococci: the nature of the problem and an agenda for the future. Emerg. Infect. Dis. 4:239-249[Medline].

11. Isenmann, R., M. Schwarz, E. Rozdzinski, R. Marre, and H. G. Beger. 2000. Aggregation substance promotes colonic mucosal invasion of Enterococcus faecalis in an ex vivo model. J. Surg. Res. 89:132-138[CrossRef][Medline].

12. Khazanie, R. 1996. Statistics in a world of applications, p 460. HarperCollins Publishers, Inc., New York, N.Y.

13. Kreft, B., R. Marre, U. Schramm, and R. Wirth. 1992. Aggregation substance of Enterococcus faecalis mediates adhesion to cultured renal tubular cells. Infect. Immun. 60:25-30[Abstract/Free Full Text].

14. Lee, M. H., N. Kosuk, J. Bailey, B. Traxler, and C. Manoil. 1999. Analysis of F factor TraD membrane topology by use of gene fusions and trypsin-sensitive insertions. J. Bacteriol. 181:6108-6113[Abstract/Free Full Text].

15. Manoil, C., and J. Bailey. 1997. A simple screen for permissive sites in proteins: analysis of Escherichia coli lac permease. J. Mol. Biol. 267:250-263[CrossRef][Medline].

16. Manoil, C., and B. Traxler. 2001. Insertion of in-frame sequence tags into proteins using transposons. Methods 20:55-61.

17. McCormick, J., H. Hirt, G. M. Dunny, and P. M. Schlievert. 2000. Pathogenic mechanisms of enterococcal endocarditis. Curr. Infect. Dis. Rep. 2:315-321[Medline].

18. McCormick, J. K., H. Hirt, C. M. Waters, T. J. Tripp, G. M. Dunny, and P. M. Schlievert. 2001. Antibodies to a surface-exposed, N-terminal domain of aggregation substance are not protective in the rabbit model of Enterococcus faecalis infective endocarditis. Infect. Immun. 69:3305-3314[Abstract/Free Full Text].

19. McMahon, C. W., B. Traxler, M. E. Grigg, and A. M. Pullen. 1998. Transposon-mediated random insertions and site-directed mutagenesis prevent the trafficking of a mouse mammary tumor virus superantigen. Virology 243:354-365[CrossRef][Medline].

20. Muscholl-Silberhorn, A. 1998. Analysis of the clumping-mediating domain(s) of sex pheromone plasmid pAD1-encoded aggregation substance. Eur. J. Biochem. 258:515-520[Medline].

21. Muscholl-Silberhorn, A. 1999. Cloning and functional analysis of Asa373, a novel adhesin unrelated to the other sex pheromone plasmid-encoded aggregation substances of Enterococcus faecalis. Mol. Microbiol. 34:620-630[CrossRef][Medline].

22. Nelson, B. D., C. Manoil, and B. Traxler. 1997. Insertion mutagenesis of the lac repressor and its implications for structure-function analysis. J. Bacteriol. 179:3721-3728[Abstract/Free Full Text].

23. Nelson, B. D., and B. Traxler. 1998. Exploring the role of integral membrane proteins in ATP-binding cassette transporters: analysis of a collection of MalG insertion mutants. J. Bacteriol. 180:2507-2514[Abstract/Free Full Text].

24. O'Sullivan, D. J., and T. R. Klaenhammer. 1993. High- and low-copy-number Lactococcus shuttle cloning vectors with features for clone screening. Gene 137:227-231[CrossRef][Medline].

25. Olmsted, S. B., G. M. Dunny, S. L. Erlandsen, and C. L. Wells. 1994. A plasmid-encoded surface protein on Enterococcus faecalis augments its internalization by cultured intestinal epithelial cells. J. Infect. Dis. 170:1549-1556[Medline].

26. Olmsted, S. B., S. M. Kao, L. J. van Putte, J. C. Gallo, and G. M. Dunny. 1991. Role of the pheromone-inducible surface protein Asc10 in mating aggregate formation and conjugal transfer of the Enterococcus faecalis plasmid pCF10. J. Bacteriol. 173:7665-7672[Abstract/Free Full Text].

27. Rakita, R. M., N. N. Vanek, K. Jacques-Palaz, M. Mee, M. M. Mariscalco, G. M. S. Dunny, W. B. Van Winkle, and S. I. Simon. 1999. Enterococcus faecalis bearing aggregation substance is resistant to killing by human neutrophils despite phagocytosis and neutrophil activation. Infect. Immun. 67:6067-6075[Abstract/Free Full Text].

28. Rosenberg, M., D. Gutnick, and E. Rosenberg. 1980. Adherence of bacteria to hydrocarbons: a Simple method for measuring cell-surface hydrophobicity. FEMS Microbiol. Lett. 9:29-33[CrossRef].

29. Ruoslahti, E. 1996. RGD and other recognition sequences for integrins. Annu. Rev. Cell Dev. Biol. 12:697-715[CrossRef][Medline].

30. Sartingen, S., E. Rozdzinski, A. Muscholl-Silberhorn, and R. Marre. 2001. Aggregation substance increases adherence and internalization, but not translocation, of Enterococcus faecalis through different intestinal epithelial cells in vitro. Infect. Immun. 68:6044-6047[Abstract/Free Full Text].

31. Schlievert, P. M., P. J. Gahr, A. P. Assimacopoulos, M. M. Dinges, J. A. Stoehr, H. Hirt, and G. M. Dunny. 1998. Aggregation and binding substances enhance pathogenicity in rabbit models of Enterococcus faecalis endocarditis. Infect. Immun. 66:218-223[Abstract/Free Full Text].

32. Snyder, W. B., and T. J. Silhavy. 1995. $beta$ -Galactosidase is inactivated by intermolecular disulfide bonds and is toxic when secreted to the periplasm of Escherichia coli. J. Bacteriol. 177:953-963[Abstract/Free Full Text].

33. Sussmuth, S. D., A. Muscholl-Silberhorn, R. Wirth, M. Susa, and R. Marre. 2000. Aggregation substance promotes adherence, phagocytosis, and intracellular survival of Enterococcus faecalis within human macrophages and suppresses respiratory burst. Infect. Immun. 68:4900-4906[Abstract/Free Full Text].

34. Trotter, K. M., and G. M. Dunny. 1990. Mutants of Enterococcus faecalis deficient as recipients in mating with donors carrying pheromone-inducible plasmids. Plasmid 24:57-67[CrossRef][Medline].

35. Vanek, N. N., S. I. Simon, K. Jacques-Palaz, M. M. Mariscalco, G. M. Dunny, and R. M. Rakita. 1999. Enterococcus faecalis aggregation substance promotes opsonin-independent binding to human neutrophils via a complement receptor type 3-mediated mechanism. FEMS Immunol. Med. Microbiol. 26:49-60[Medline].

36. Wirth, R. 1994. The sex pheromone system of Enterococcus faecalis. More than just a plasmid-collection mechanism? Eur. J. Biochem. 222:235-246[Medline].

37. Wirth, R., F. Y. An, and D. B. Clewell. 1986. Highly efficient protoplast transformation system for Streptococcus faecalis and a new Escherichia coli-S. faecalis shuttle vector. J. Bacteriol. 165:831-836[Abstract/Free Full Text].

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1.	Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl. 1990. Current protocols in molecular biology. John Wiley & Sons, Inc., New York, N.Y.
2.	Bae, T., S. Clerc-Bardin, and G. M. Dunny. 2000. Analysis of expression of prgX, a key negative regulator of the transfer of the Enterococcus faecalis pheromone-inducible plasmid pCF10. J. Mol. Biol. 297:861-875[CrossRef][Medline].
3.	Bryan, E. M., T. Bae, H. Kleerebezem, and G. M. Dunny. 2000. Improved vectors for nisin-controlled expression in gram-positive bacteria. Plasmid 44:183-190[CrossRef][Medline].
4.	Chow, J. W., L. A. Thal, M. B. Perri, J. A. Vazquez, S. M. Donabedian, and D. B. Clewell. 1993. Plasmid-associated hemolysin and aggregation substance production contribute to virulence in experimental enterococcal endocarditis. Antimicrob. Agents Chemother. 37:2474-2477[Abstract/Free Full Text].
5.	Christie, P. J., and G. M. Dunny. 1986. Identification of regions of the Streptococcus faecalis plasmid pCF-10 that encode antibiotic resistance and pheromone response functions. Plasmid 15:230-241[CrossRef][Medline].
6.	Dunny, G. M., B. L. Brown, and D. B. Clewell. 1978. Induced cell aggregation and mating in Streptococcus faecalis: evidence for a bacterial sex pheromone. Proc. Natl. Acad. Sci. USA 75:3479-3483[Abstract/Free Full Text].
7.	Galli, D., F. Lottspeich, and R. Wirth. 1990. Sequence analysis of Enterococcus faecalis aggregation substance encoded by the sex pheromone plasmid pAD1. Mol. Microbiol. 4:895-904[CrossRef][Medline].
8.	Hirt, H., S. L. Erlandsen, and G. M. Dunny. 2000. Heterologous inducible expression of Enterococcus faecalis pCF10 aggregation substance Asc10 in Lactococcus lactis and Streptococcus gordonii contributes to cell hydrophobicity and adhesion to fibrin. J. Bacteriol. 182:2299-2306[Abstract/Free Full Text].
9.	Hirt, H., G. Wanner, D. Galli, and R. Wirth. 1993. Biochemical, immunological and ultrastructural characterization of aggregation substances encoded by Enterococcus faecalis sex-pheromone plasmids. Eur. J. Biochem. 211:711-716[Medline].
10.	Huycke, M. M., D. F. Sahm, and M. S. Gilmore. 1998. Multiple-drug resistant enterococci: the nature of the problem and an agenda for the future. Emerg. Infect. Dis. 4:239-249[Medline].
11.	Isenmann, R., M. Schwarz, E. Rozdzinski, R. Marre, and H. G. Beger. 2000. Aggregation substance promotes colonic mucosal invasion of Enterococcus faecalis in an ex vivo model. J. Surg. Res. 89:132-138[CrossRef][Medline].
12.	Khazanie, R. 1996. Statistics in a world of applications, p 460. HarperCollins Publishers, Inc., New York, N.Y.
13.	Kreft, B., R. Marre, U. Schramm, and R. Wirth. 1992. Aggregation substance of Enterococcus faecalis mediates adhesion to cultured renal tubular cells. Infect. Immun. 60:25-30[Abstract/Free Full Text].
14.	Lee, M. H., N. Kosuk, J. Bailey, B. Traxler, and C. Manoil. 1999. Analysis of F factor TraD membrane topology by use of gene fusions and trypsin-sensitive insertions. J. Bacteriol. 181:6108-6113[Abstract/Free Full Text].
15.	Manoil, C., and J. Bailey. 1997. A simple screen for permissive sites in proteins: analysis of Escherichia coli lac permease. J. Mol. Biol. 267:250-263[CrossRef][Medline].
16.	Manoil, C., and B. Traxler. 2001. Insertion of in-frame sequence tags into proteins using transposons. Methods 20:55-61.
17.	McCormick, J., H. Hirt, G. M. Dunny, and P. M. Schlievert. 2000. Pathogenic mechanisms of enterococcal endocarditis. Curr. Infect. Dis. Rep. 2:315-321[Medline].
18.	McCormick, J. K., H. Hirt, C. M. Waters, T. J. Tripp, G. M. Dunny, and P. M. Schlievert. 2001. Antibodies to a surface-exposed, N-terminal domain of aggregation substance are not protective in the rabbit model of Enterococcus faecalis infective endocarditis. Infect. Immun. 69:3305-3314[Abstract/Free Full Text].
19.	McMahon, C. W., B. Traxler, M. E. Grigg, and A. M. Pullen. 1998. Transposon-mediated random insertions and site-directed mutagenesis prevent the trafficking of a mouse mammary tumor virus superantigen. Virology 243:354-365[CrossRef][Medline].
20.	Muscholl-Silberhorn, A. 1998. Analysis of the clumping-mediating domain(s) of sex pheromone plasmid pAD1-encoded aggregation substance. Eur. J. Biochem. 258:515-520[Medline].
21.	Muscholl-Silberhorn, A. 1999. Cloning and functional analysis of Asa373, a novel adhesin unrelated to the other sex pheromone plasmid-encoded aggregation substances of Enterococcus faecalis. Mol. Microbiol. 34:620-630[CrossRef][Medline].
22.	Nelson, B. D., C. Manoil, and B. Traxler. 1997. Insertion mutagenesis of the lac repressor and its implications for structure-function analysis. J. Bacteriol. 179:3721-3728[Abstract/Free Full Text].
23.	Nelson, B. D., and B. Traxler. 1998. Exploring the role of integral membrane proteins in ATP-binding cassette transporters: analysis of a collection of MalG insertion mutants. J. Bacteriol. 180:2507-2514[Abstract/Free Full Text].
24.	O'Sullivan, D. J., and T. R. Klaenhammer. 1993. High- and low-copy-number Lactococcus shuttle cloning vectors with features for clone screening. Gene 137:227-231[CrossRef][Medline].
25.	Olmsted, S. B., G. M. Dunny, S. L. Erlandsen, and C. L. Wells. 1994. A plasmid-encoded surface protein on Enterococcus faecalis augments its internalization by cultured intestinal epithelial cells. J. Infect. Dis. 170:1549-1556[Medline].
26.	Olmsted, S. B., S. M. Kao, L. J. van Putte, J. C. Gallo, and G. M. Dunny. 1991. Role of the pheromone-inducible surface protein Asc10 in mating aggregate formation and conjugal transfer of the Enterococcus faecalis plasmid pCF10. J. Bacteriol. 173:7665-7672[Abstract/Free Full Text].
27.	Rakita, R. M., N. N. Vanek, K. Jacques-Palaz, M. Mee, M. M. Mariscalco, G. M. S. Dunny, W. B. Van Winkle, and S. I. Simon. 1999. Enterococcus faecalis bearing aggregation substance is resistant to killing by human neutrophils despite phagocytosis and neutrophil activation. Infect. Immun. 67:6067-6075[Abstract/Free Full Text].
28.	Rosenberg, M., D. Gutnick, and E. Rosenberg. 1980. Adherence of bacteria to hydrocarbons: a Simple method for measuring cell-surface hydrophobicity. FEMS Microbiol. Lett. 9:29-33[CrossRef].
29.	Ruoslahti, E. 1996. RGD and other recognition sequences for integrins. Annu. Rev. Cell Dev. Biol. 12:697-715[CrossRef][Medline].
30.	Sartingen, S., E. Rozdzinski, A. Muscholl-Silberhorn, and R. Marre. 2001. Aggregation substance increases adherence and internalization, but not translocation, of Enterococcus faecalis through different intestinal epithelial cells in vitro. Infect. Immun. 68:6044-6047[Abstract/Free Full Text].
31.	Schlievert, P. M., P. J. Gahr, A. P. Assimacopoulos, M. M. Dinges, J. A. Stoehr, H. Hirt, and G. M. Dunny. 1998. Aggregation and binding substances enhance pathogenicity in rabbit models of Enterococcus faecalis endocarditis. Infect. Immun. 66:218-223[Abstract/Free Full Text].
32.	Snyder, W. B., and T. J. Silhavy. 1995. $beta$ -Galactosidase is inactivated by intermolecular disulfide bonds and is toxic when secreted to the periplasm of Escherichia coli. J. Bacteriol. 177:953-963[Abstract/Free Full Text].
33.	Sussmuth, S. D., A. Muscholl-Silberhorn, R. Wirth, M. Susa, and R. Marre. 2000. Aggregation substance promotes adherence, phagocytosis, and intracellular survival of Enterococcus faecalis within human macrophages and suppresses respiratory burst. Infect. Immun. 68:4900-4906[Abstract/Free Full Text].
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