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The Vibrio cholerae FlgM Homologue Is an Anti-²⁸ Factor That Is Secreted through the Sheathed Polar Flagellum

Department of Microbiology and Immunology, University of Texas Health Science Center, San Antonio, Texas

Received 20 February 2004/ Accepted 8 April 2004

	ABSTRACT

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Vibrio cholerae has a single polar sheathed flagellum that propels the cells of this bacterium. Flagellar synthesis, motility, and chemotaxis have all been linked to virulence in this human pathogen. V. cholerae expresses flagellar genes in a hierarchy consisting of ⁵⁴- and ²⁸-dependent transcription. In other bacteria, ²⁸ transcriptional activity is controlled by an anti-²⁸ factor, FlgM. We demonstrate that the V. cholerae FlgM homologue (i) physically interacts with ²⁸, (ii) has a repressive effect on some V. cholerae ²⁸-dependent flagellar promoters, and (iii) is secreted through the polar sheathed flagellum, consistent with anti-²⁸ activity. Interestingly, FlgM does not have a uniform repressive effect on all ²⁸-dependent promoters, as determined by measurement of ²⁸-dependent transcription in cells either lacking FlgM (flgM) or incapable of secretion (fliF). Further analysis of a fliF strain revealed that this flagellar assembly block causes a decrease in class III (FlrC- and ⁵⁴-dependent) and class IV (²⁸-dependent), but not class II (FlrA- and ⁵⁴-dependent), flagellar transcription. V. cholerae flgM and fliA (encodes ²⁸) mutants were only modestly affected in their ability to colonize the infant mouse intestine, a measure of virulence. Our results demonstrate that V. cholerae FlgM functions as an anti-²⁸ factor and that the sheathed flagellum is competent for secretion of nonstructural proteins.

	INTRODUCTION

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Studies of bacterial flagellar assembly have revealed that the flagellum is assembled in a stepwise fashion that begins by insertion of a type III export apparatus into the cytoplasmic membrane (reviewed in reference 27). Flagellar components are then secreted through this export machinery to be added to the growing tip of the flagellum in the specific order in which they are assembled (reviewed in reference 42). The bulk of the flagellum is composed of flagellin subunits, which are only added to the flagellum after the basal-body-hook structure is completed. Transcription of flagellar genes generally occurs in a hierarchical fashion that mirrors assembly of the nascent flagellum; i.e., the genes encoding early flagellar components are transcribed prior to the genes encoding late flagellar components, such as flagellin subunits (24; reviewed in reference 41).

In Salmonella enterica serovar Typhimurium, transcription of the flagellin gene is repressed until the basal-body-hook structure is completed, through the action of an anti-sigma factor, FlgM. The flagellin gene is transcribed by RNA polymerase (RNAP) containing the alternate sigma factor ²⁸ (encoded by fliA) (34). FlgM binds to ²⁸ and prevents its association with RNAP, preventing flagellin gene transcription (23). However, once the basal-body-hook structure is assembled, FlgM is secreted through the flagellar export apparatus to the extracellular milieu, which allows ²⁸ to associate with RNAP and transcribe the flagellin gene (15). Thus, the function of FlgM is to couple flagellar assembly to appropriate temporal flagellar gene transcription.

Flagellar gene transcription in Vibrio cholerae, which possesses a single polar sheathed flagellum, is also organized into a transcription hierarchy (35). However, the four-tiered transcription hierarchy has notable differences from the three-tiered hierarchy of S. enterica serovar Typhimurium, which possess multiple peritrichous flagella. In V. cholerae, the genes encoding the early structural components of the flagellum (basal-body-hook) are transcribed in two distinct temporal classes (II and III) by RNAP containing the alternate sigma factor ⁵⁴; in contrast, transcription of the equivalent genes in S. enterica serovar Typhimurium occurs within the single "early" temporal class (II) by RNAP containing the housekeeping ⁷⁰ subunit. However, the last temporal class of flagellar genes in V. cholerae (class IV), as in S. enterica serovar Typhimurium (class III), is transcribed by RNAP containing ²⁸. The main ²⁸-dependent genes are four distinct flagellin genes, flaB, flaC, flaD, and flaE (20, 35). ⁵⁴-dependent transcription of a fifth flagellin gene, flaA, precedes transcription of the other four flagellin genes (20). The four-tiered ⁵⁴- and ²⁸-dependent flagellar transcription hierarchy of V. cholerae (35) is likely to be identical to the polar hierarchy of V. parahaemolyticus (18), is remarkably similar to those of Pseudomonas aeruginosa (3) and Campylobacter jejuni (14), and has similarities to that of Helicobacter pylori (1), suggesting that this flagellar hierarchy may be common among gram-negative bacteria with polar flagella.

The ⁵⁴-dependent FlaA flagellin is essential for V. cholerae motility and flagellar synthesis, while the ²⁸-dependent FlaB, FlaC, FlaD, and FlaE flagellins are largely dispensable both singly and in combination (20). A fliA strain (lacking ²⁸) is nonmotile and does not transcribe flaB, flaC, flaD, or flaE but produces a truncated flagellum, indicating that some FlaA subunits are assembled (35). Because FlaA transcription and assembly into the flagellum appear to precede the transcription and incorporation of the other flagellin subunits, it suggests that the checkpoint that controls ²⁸-dependent transcription may differ between V. cholerae and S. enterica serovar Typhimurium, where completion of the basal-body-hook structure causes the export of FlgM and ²⁸-dependent transcription (17). Also, the presence of a sheath enveloping the V. cholerae flagellum, which is contiguous with the outer membrane (7), could inhibit or prevent the secretion of nonstructural proteins, such as an anti-sigma factor, through the flagellum; S. enterica serovar Typhimurium flagella are not sheathed. These observations invited the question of whether V. cholerae FlgM functions similarly to FlgM of S. enterica serovar Typhimurium.

FlgM homologues have been identified and characterized in the gram-negative polar flagellates H. pylori (1, 16) and P. aeruginosa (6). These studies demonstrated that the FlgM homologues in these bacteria physically interact with ²⁸ and inhibit ²⁸-dependent transcription, but they did not address the question of whether FlgM is secreted through the flagellum. In fact, Josenhans et al. suggested that FlgM is not secreted through the sheathed H. pylori flagellum (16). A report on a flgM C. jejuni mutant (14) demonstrated that the FlgM of that organism has only weak repressive activity on ²⁸-dependent transcription but also did not address FlgM secretion. We report here that the V. cholerae FlgM homologue has the characteristics of the S. enterica serovar Typhimurium anti-²⁸ factor: it physically interacts with ²⁸, it represses transcription from some ²⁸-dependent promoters, and it is secreted through the (polar sheathed) flagellum.

	MATERIALS AND METHODS

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Bacterial strains and media. Escherichia coli strain DH5 (11) was used for cloning manipulations, SM10pir (32) was used to transfer plasmids to V. cholerae by conjugation, and BL21(DE3) (Novagen) was used for protein expression. The V. cholerae strains used in this study are listed in Table 1. Construction of chromosomal deletions and insertions with pKEK229, a pCVD442 derivative with the sacB gene (4), has been described previously (2). Bacteriophage CP-T1ts-mediated transduction (12) was used to construct KKV1441(flgM::Cm^r); the correct construction of all strains was verified by PCR and sequencing.

Plasmid construction. All of the plasmids and oligonucleotide primers used are listed in Table 1. V. cholerae O395 chromosomal DNA was used as the template for PCR amplification. The in-frame deletion in flgM (flgM) was constructed by first amplifying the 5' fragment with oligonucleotides FLGMDEL1 and FLGMDEL2, digesting the amplified product with EcoRI and BamHI, and then ligating it into similarly digested pWSK30 (39) to form pKEK375. The 3' fragment was PCR amplified with oligonucleotides FLGMDEL3 and FLGMDEL4, digested with EcoRI and HindIII, and ligated into similarly digested pKEK375 to form pKEK381 (flgM). This results in the removal of 165 nucleotides that correspond to amino acids 29 to 83 of the predicted gene product. The chloramphenicol acetyltransferase gene from pACYC184 (37) was amplified by PCR with primers CAT1 and CAT2 (22), digested with MfeI, and ligated into pKEK381 digested with EcoRI to form pKEK411 (flgM::Cm^r). The flgM and flgM::Cm^r mutations were moved into plasmid pKEK229 via NotI and SalI digestion and ligation to form pKEK389 and pKEK427, respectively.

To construct a plasmid for the expression of FlgM with an amino-terminal FLAG tag (FLAG-FlgM), flgM was PCR amplified with primers FLAGFLGM and FLGMUBAMHI, digested with NcoI and BamHI, and ligated into similarly digested pET15b (Novagen) to form pKEK460. pKEK460 was then digested with PshAI and HindIII and ligated with a PshAI-HindIII fragment of pACYC184 (37) to generate pKEK470. This plasmid still contains the T7lac promoter and FLAG-FlgM, but with p15A ori and Cm^r from pACYC184. For expression of FLAG-FlgM in V. cholerae, pKEK470 was digested with NcoI and HindIII and ligated into similarly digested pBAD24 (10) to form pKEK474. The plasmid used for expression of ²⁸ with an amino-terminal His₆ tag (His-²⁸) was constructed by PCR amplification of fliA with primers FLIANDEI and FLIAUBAMHI, followed by digestion with NdeI and BamHI and ligation into similarly digested pET-15b to form pKEK462.

ß-Galactosidase assays. V. cholerae strains were transformed with the promoter-lacZ fusion-containing plasmids listed in Table 1, grown in LB plus antibiotic, and then harvested at an optical density at 600 nm of 0.2 to 0.4. Bacterial cells were permeabilized with chloroform and sodium dodecyl sulfate (SDS) and assayed for ß-galactosidase activity by the method of Miller (31). All experiments were performed at least three separate times.

Electron microscopy. Strains were grown to mid-log phase in LB, centrifuged, and then resuspended in 0.15 M NaCl. Samples were allowed to adhere to a carbon-coated grid and stained with 1% uranyl acetate before microscopy with a JEOL 1230 microscope. The AMT software was used to measure the lengths of flagella on wild-type and flgM mutant V. cholerae strains (25 of each), which were determined to be significantly different by Student's two-tailed t test.

In vivo colonization assays. The infant mouse colonization assay has been described previously (9). The inocula consisted of 10⁶ CFU for both wild-type and mutant bacteria.

Protein detection. For coprecipitation of His-²⁸ and FLAG-FlgM, plasmids pKEK470 and/or pKEK462 were transformed into BL21(DE3) and expression of the proteins was induced by growth in LB with 1 mM isopropyl-ß-D-thiogalactopyranoside (IPTG) for 5 h at 37°C. Supernatants of sonicated cells were mixed with anti-His Dynabeads (Dynal Biotech), pelleted, and eluted in accordance with the manufacturer's instructions.

For detection of FLAG-FlgM secretion, KKV598 (wild type) and KKV1247 (fliF) were transformed with pKEK474. These strains were grown in LB plus 0.1% arabinose at 37°C for 2 h. Samples were removed and centrifuged at 17,000 x g for 30 min. The supernatants were passed through a 0.2-µm syringe filter and concentrated with 10% trichloroacetic acid (TCA). Samples were then centrifuged (68,000 x g for 1.5 h), and the pellets were washed twice with cold acetone.

Samples were separated by SDS-15% polyacrylamide gel electrophoresis, probed by Western immunoblotting with either His-Tag (Novagen) or anti-FLAG M2 (Sigma) monoclonal antibody, and detected with ECL detection reagent (Amersham-Pharmacia).

	RESULTS

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Interaction of FlgM with ²⁸. The gene encoding a FlgM homologue was identified in the V. cholerae genome sequence (VC2204) (13). The flgM gene is predicted to encode a protein of 11.3 kDa. As we noted previously (35), V. cholerae FlgM has homology with S. enterica serovar Typhimurium FlgM (28% identity). If V. cholerae FlgM functions as an anti-²⁸ factor, it is predicted to physically interact with ²⁸ (FliA). To detect a physical interaction between FlgM and ²⁸, His-tagged V. cholerae ²⁸ and FLAG-tagged V. cholerae FlgM were coexpressed from different compatible plasmids within E. coli (Fig. 1). Magnetic metal chelation beads (anti-His; Dynal Biotech) were then used to precipitate His-²⁸ from the E. coli lysate. Eluates from the magnetic beads were separated by SDS-polyacrylamide gel electrophoresis and then probed with either anti-His or anti-FLAG antibodies by Western immunoblotting.

View larger version (44K): [in this window] [in a new window]   FIG. 1. Interaction of V. cholerae FlgM with 28. His-28 and FLAG-FlgM were expressed separately and together in E. coli BL21(DE3), which contains T7 polymerase, from T7 promoters in plasmids pKEK462 and pKEK470, respectively, and magnetic anti-His beads (Dynal Biotech) were used to capture His-tagged protein from cell lysates as described in Materials and Methods. In the upper panel, samples were separated on Coomassie-stained polyacrylamide gel, and the lower panels show Western immunoblots of these same samples probed with anti-His tag and anti-FLAG tag antibodies. Masses of molecular size markers are noted on the left in kilodaltons, and arrows depict migration of His-28 and FLAG-FlgM. Lane numbers correspond to BL21(DE3) cells expressing His-28 (lane 1, whole-cell lysate; lane 2, anti-His bead eluate), FLAG-FlgM (lane 3, whole-cell lysate, lane 4, anti-His bead eluate), and His-28 and FLAG-FlgM (lane 5, whole-cell lysate, lane 6, anti-His bead eluate).

Secretion of FlgM through the V. cholerae flagellum. The S. enterica serovar Typhimurium FlgM protein is secreted through the flagellar export apparatus. To monitor secretion of V. cholerae FlgM through the flagellar export apparatus, a FLAG tag was fused to the N terminus of FlgM to facilitate detection; a FLAG tag at the N terminus of S. enterica serovar Typhimurium FlgM does not inhibit secretion through the flagellum (K. Hughes, personal communication). To determine if the V. cholerae FlgM protein is likewise secreted through the flagellum, the FLAG-FlgM protein was expressed in a wild-type (flagellated) V. cholerae strain. FLAG-FlgM was also expressed within a fliF V. cholerae strain, which lacks the MS ring, the first component assembled in the flagellum, and thus this strain lacks any flagellar structure or export apparatus. Protein in the filtered supernatant was concentrated by TCA precipitation, separated by SDS-polyacrylamide gel electrophoresis, and then subjected to Western immunoblot analysis with anti-FLAG antibodies.

FLAG-FlgM could be detected both in the supernatant (S) and in the cell pellet (P) of the wild-type (flagellated) strain (WT, Fig. 2). However, FLAG-FlgM was only found within the cell pellet (P) of the fliF (nonflagellated) strain (fliF) and there was no detectable FLAG-FlgM present in the supernatant (S). These results indicate that there is a requirement for the flagellum to achieve secretion of FlgM into the supernatant, consistent with FlgM secretion through the V. cholerae polar (sheathed) flagellum. Interestingly, the FlgM protein in the supernatant has a slightly different mobility in the gel than the FlgM protein within the cells, suggesting either some C-terminal processing or an SDS-resistant conformational change.

View larger version (30K): [in this window] [in a new window]   FIG. 2. FlgM is secreted through the V. cholerae flagellum. FLAG-FlgM was expressed from plasmid pKEK474 in V. cholerae strains KKV598 (wild type [WT]) and KKV1247 (fliF mutant). Bacterial pellets (P) and supernatants (S) were processed for Western immunoblot analysis with anti-FLAG antibodies as described in Materials and Methods.

To obtain a fliA⁺ strain with the flgM mutation, we first constructed a flgM::Cm^r chromosomal mutation in fliA mutant strain KKV1113 via suicide plasmid pKEK427 (strain KKV1365) and then moved the flgM::Cm^r mutation into the wild-type (fliA⁺) strain (KKV1441) via CP-T1ts-mediated transduction (12). Cm^r transductants in the fliA⁺ background took 2 days to form colonies on plates, compared to Cm^r transductants in the fliA mutant background, which only took 1 day to form colonies. PCR analysis demonstrated that these Cm^r transductants had a chromosomal flgM::Cm^r mutation (not shown). The flgM::Cm^r mutation was then replaced with flgM (without any insertion) via suicide plasmid pKEK389. In this manner we constructed flgM mutant V. cholerae strain KKV1461. Interestingly, although the flgM strain took 2 days to form colonies on selective plates, its growth curve is indistinguishable from that of the wild-type strain in liquid LB (not shown).

Motility of the flgM mutant strain was measured in motility agar plates (Fig. 3A). The swimming pattern of this strain was slightly reduced compared to that of the wild-type strain, indicating that the flgM mutation has a modest negative effect on the ability of the bacteria to swim from the point of inoculation in this assay. In contrast, the fliA mutation abolished motility, as we have shown previously (35). A fliF mutant strain, which contains a mutation in the structural gene for the MS ring, the first component of the flagellum assembled (27), is also nonmotile in this assay, as expected. A flgM mutant of P. aeruginosa showed a significant motility defect in this assay (6), suggesting possible differences between the function of V. cholerae FlgM and that of P. aeruginosa FlgM.

View larger version (136K): [in this window] [in a new window]   FIG. 3. Motility phenotype and electron micrograph of a V. cholerae flgM strain. (A) V. cholerae strains KKV598 (wild type [WT]), KKV1114 (fliA mutant), KKV1461 (flgM mutant), and KKV1247 (fliF mutant) were inoculated into motility agar and incubated at 30°C. Electron micrographs of V. cholerae strains KKV598 (wild type) (B) and KKV1461 (flgM) (C) are also shown. Bars are equivalent to 2 µm.

FlgM has repressive effects on ²⁸-dependent transcription. If FlgM functions as an anti-²⁸ factor, its absence in a flgM mutant would be predicted to cause an increase in ²⁸-dependent transcription. Transcription of the five V. cholerae flagellins was measured by promoter-lacZ transcriptional fusion plasmids (20) in the wild-type, fliA, flgM, and fliA flgM strains (Fig. 4). The flaA promoter is a ⁵⁴-dependent class III promoter, while the flaB, flaC, flaD, and flaE promoters are ²⁸-dependent class IV promoters (35).

View larger version (16K): [in this window] [in a new window]   FIG. 4. Expression of flagellin promoters in fliA and flgM mutant V. cholerae strains. V. cholerae strains KKV598 (wild type), KKV113 (fliA mutant), KKV1461 (flgM mutant), and KKV1384 (fliA flgM mutant) carrying plasmids pKEK80 (flaAp-lacZ), pKEK79 (flaBp-lacZ), pKEK76 (flaCp-lacZ), pKEK77 (flaDp-lacZ), and pKEK81 (flaEp-lacZ) were assayed for ß-galactosidase activity during logarithmic growth in LB. Assays were performed in triplicate, and standard deviations are shown.

Lack of the MS ring causes decreases in class III and IV and increases in class II flagellar transcription. Because the MS ring is the first structural component assembled in the nascent flagellum (27), absence of the MS ring in a fliF V. cholerae mutant will prevent export and subsequent assembly of any flagellar component located exterior to the cytoplasm. To determine the effect on transcription of blocking flagellar assembly at the initial step, we measured the transcription of a number of class II, III, and IV promoters in the V. cholerae wild-type and fliF mutant strains (Fig. 5).

View larger version (26K): [in this window] [in a new window]   FIG. 5. Expression of class II, III, and IV flagellar promoters in a fliF mutant V. cholerae strain. V. cholerae strains KKV598 (wild type) and KKV1247 (fliF mutant) carrying plasmids pKEK72 (flrBp-lacZ), pKEK327 (fliEp-lacZ), pKEK329 (flhAp-lacZ), pKEK332 (flgBp-lacZ), pKEK331 (flgKp-lacZ), pKEK80 (flaAp-lacZ), pKEK415 (flaGp-lacZ), pKEK79 (flaBp-lacZ), pKEK76 (flaCp-lacZ), pKEK77 (flaDp-lacZ), and pKEK81 (flaEp-lacZ) were assayed for ß-galactosidase activity during logarithmic growth in LB. Assays were performed in triplicate, and standard deviations are shown.

flgM and fliA have little effect on intestinal colonization. Flagellar synthesis, regulation, and chemotaxis have all been linked to V. cholerae colonization defects in the infant mouse (2, 26, 40), but the connection between these phenomena remains unclear. To determine the effect of flgM and fliA mutations on V. cholerae intestinal colonization of the infant mouse, a competition assay was performed with an inoculum that consisted of both mutant and isogenic wild-type strains (see Materials and Methods). Colonization defects are recognized by a competitive index (CI) of less than 1.

The fliA, flgM, and fliA flgM mutant strains demonstrated modest colonization defects in this assay (Fig. 6). The fliA and fliA flgM mutant strains were more affected for colonization (CI, 0.3) than the flgM strain (CI, 0.601), indicating that loss of ²⁸ is more deleterious for colonization than is loss of FlgM. Still, these are modest colonization defects, demonstrating that ²⁸ and FlgM play little role in intestinal colonization. Control experiments showed wild-type growth rates of all strains in LB at 37°C; thus, no obvious in vitro growth defects account for the modest in vivo colonization defects of these strains.

View larger version (13K): [in this window] [in a new window]   FIG. 6. Intestinal colonization of fliA and flgM mutant V. cholerae strains. Strains KKV1113 (fliA mutant), KKV1461 (flgM mutant), and KKV1384 (fliA flgM mutant) were coinoculated with O395 perorally into infant mice at a ratio of 1:1; intestinal homogenates were recovered at 24 h postinoculation, and CFU of wild-type and mutant strains were counted. The CI is given as the output mutant/wild-type ratio divided by the input mutant/wild-type ratio; each value shown is from an individual mouse.

	DISCUSSION

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V. cholerae possesses a single polar sheathed flagellum that contains five distinct flagellin subunits; four of the flagellin genes are transcribed by ²⁸ holoenzyme, while a fifth flagellin gene is transcribed by ⁵⁴ holoenzyme (20). Transcription and assembly of the ⁵⁴-dependent flagellin, FlaA, appear to precede transcription and assembly of the ²⁸-dependent flagellins (35). This situation differs from that in S. enterica serovar Typhimurium, where there is a single flagellin gene transcribed by ²⁸ holoenzyme upon completion of the basal-body-hook structure, suggesting that control of ²⁸-dependent transcription differs between V. cholerae and S. enterica serovar Typhimurium. Also, the V. cholerae flagellum, unlike those of S. enterica serovar Typhimurium, is covered by a sheath that may impede the secretion of nonstructural proteins, such as FlgM.

Our results demonstrate that V. cholerae FlgM interacts with ²⁸, is secreted through the flagellum, can inhibit transcription of some ²⁸-dependent promoters, and represses flagellar length; all of these functions are consistent with anti-²⁸ activity, as initially characterized in S. enterica serovar Typhimurium. One would therefore anticipate that the absence of FlgM would result in increased ²⁸-dependent transcription at all of the ²⁸-dependent flagellin promoters, and in fact flaD and flaE transcription increased in the flgM strain. However, flaC transcription actually decreased in a flgM strain while flaB transcription was unaffected. Perhaps unregulated ²⁸ activity causes sequestration of a limited amount of ²⁸ holoenzyme at certain promoters (flaD, flaE), causing a decrease in transcription at other promoters (flaC).

It is difficult to rationalize the unresponsiveness of the flaB promoter to both the absence of FlgM and the absence of the MS ring. This promoter is clearly ²⁸ dependent, yet its activity is not diminished in the absence of secretion (fliF mutant) nor increased in the absence of FlgM; thus, this promoter behaves differently than other ²⁸- and FlgM-controlled promoters. These differences in transcriptional responsiveness of the individual flagellin genes undoubtedly lead to differences in the composition of the flagellin subunits within the flagellum under different conditions, and we predict that this leads to altered swimming behavior. Complex flagella (i.e., composed of multiple distinct flagellin subunits) are present in many bacteria with polar flagella (e.g., Vibrio, Pseudomonas, and Campylobacter spp., etc.), but no studies have been performed yet that link the flagellin composition under different conditions to specific attributes of flagellar performance, such as rotation rate, speed, etc.

The lack of the MS ring in V. cholerae (fliF mutant) led to general decreases in class III and IV flagellar transcription. We have already shown that transcription of class III genes is dependent on phosphorylation of FlrC (encoded by a class II gene) (2, 21), which suggests that the lack of secretion and/or lack of the MS ring inhibits phosphorylation of FlrC. Although FlrB, the kinase that phosphorylates FlrC, has been identified (2), it is not clear what modulates FlrB activity; these results suggest that it may be either an early structural component or a functional secretion apparatus. Transcription of the analogous C. jejuni class III genes, which are regulated by a FlrC homologue, FlgR, have been shown to depend upon the formation of the flagellar secretory apparatus (14), so we favor a similar functional, rather than structural, checkpoint in V. cholerae.

Although a number of bacteria possess sheathed flagella (e.g., Vibrio and Helicobacter spp.), very little is known about the sheath itself. The sheath is hypothesized to mask the proinflammatory flagellin subunits from the host immune system (28). Limited studies of V. cholerae demonstrated that the sheath possesses lipopolysaccharide, indicating that it is contiguous with the outer membrane (7). Additional studies of V. alginolyticus and V. anguillarum have identified a specific protein and lipopolysaccharide associated with the flagellar sheath in these species (8, 33). Analysis of mutations in hook-associated proteins that connect the flagellin filaments to the basal body in V. parahaemolyticus suggested that the sheath acts as a barrier to the secretion of flagellin subunits to the extracellular milieu (29), raising the question of the competence of the sheathed Vibrio flagellum to secrete FlgM (28).

Our studies demonstrate that V. cholerae FlgM is secreted through the sheathed flagellum, thus opening up the possibility that other nonstructural proteins could also be secreted through the flagellar export machinery. Type III secretion systems (TTSS) are frequently used by pathogenic bacteria to alter host physiology during infection, but the only TTSS present in the V. cholerae genome is the flagellar export apparatus (13). However, Yersinia enterocolitica is known to use the flagellar TTSS to secrete a virulence-associated phospholipase (43). Various studies have linked motility and flagellar synthesis to aspects of V. cholerae virulence (2, 5, 9, 26, 36, 40), but the phenomena are frequently strain and animal model dependent so it has been difficult to elucidate the contribution of the flagellum to cholera pathogenesis. The studies presented here demonstrate that the lack of ²⁸ and/or FlgM has a modest impact on the ability of a classical V. cholerae strain (O395) to colonize the infant mouse intestine; this animal model has been useful in predicting colonization behavior in humans (19). The effect of these mutations in other V. cholerae strains and on other aspects of virulence (intoxication, dissemination, reactogenicity, etc.) may be more profound.

	ACKNOWLEDGMENTS

 
We thank Kelly Hughes for helpful discussions.

This work was supported by NIH AI43486 to K.E.K.

	FOOTNOTES

 
* Corresponding author. Mailing address: Department of Biology, University of Texas San Antonio, 6900 N. Loop 1604 West, San Antonio, TX 78249-0662. Phone: (210) 458-6140. Fax: (210) 458-5658. E-mail: klose{at}utsa.edu.

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