Source: http://www.kpubs.org/article/articleMain.kpubs?articleANo=E1HKAL_2011_v14n2_73
Timestamp: 2019-04-21 00:18:59+00:00

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Vibrio parahaemolyticus possesses two flagella systems: polar and lateral flagella for swimming in liquid and swarming on solid surfaces or in viscous environments. To elucidate the pathogenic role of these dual flagella systems, we constructed single- and double-deletion mutants of the lafA and flhAB flagellum genes and investigated their biofilm formation, cell adhesion, and colonization of the small intestine of suckling mice. The double-mutant strain was more impaired in biofilm formation than either of the single-mutant strains. In addition, the lafA, flhAB, and double-mutant strains showed 40%, 45%, and 60%, respectively, lower adherence to HeLa cells than the wild-type strain. Moreover, the lafA, flhAB, and double-mutant strains exhibited 49%,5.6 and 6.7 times, respectively, lower colonization in a competition assay than the wild-type strain. These findings indicated that polar flagella were more important than lateral flagella for the pathogenesis of V. parahaemolyticus.
To adapt and survive under changing environmental conditions, bacteria can modulate their gene expression and direct their movements by various processes such as flagella-mediated chemotaxis. Vibrio parahaemolyticus is a Gram-negative bacterium that possesses two types of flagella on swimmer and swarmer cells, namely, polar and lateral flagella, which are used to swim in liquids and swarm on solid surfaces or in viscous environments,respectively (McCarter, 2004). Swimmer cells are rod-shaped, about 2 ㎛ long, and have a single polar flagellum, while swarmer cells are multinucleate,more than 30 ㎛ long, and have many lateral flagella(Shinoda et al., 1974; McCarter and Silverman, 1990).Polar flagella are formed constitutively, whereas lateral flagella are induced under conditions that disable the polar flagella, such as on solid surfaces, in viscous environments (McCarter et al., 1988), and in the presence of phenamil, a potent inhibitor of sodium ion channels (Klose and Mekalanos, 1998)that disrupt the sodium-motive force that powers flagella (Atsumi et al., 1992). Furthermore, the swimmer and swarmer cell types can reversibly differentiate in different environments. For example,the synthesis of lateral flagella ceases when the environment changes from solid to liquid (Stewart and McCarter, 2003). More generally, the lateral flagella of V. parahaemolyticus form in response to changes in environmental factors, such as pH,temperature, and NaCl concentration (Belas and Colwell, 1982).
In V. parahaemolyticus , 60 polar flagellum genes are located exclusively on the large chromosome,whereas 38 lateral flagellum genes are found in two regions of the small chromosome (Makino et al.,2003; Stewart and McCarter, 2003). In addition,several regulatory genes, such as the scrABC operon,control the formation of lateral flagella (Boles and McCarter, 2002). For example, LafK and FliAL control the expression of early and late genes of the lateral flagellum of V. parahaemolyticus (Stewart and McCarter, 2003).
Recently, we reported that VpaH, which encodes a novel H-NS-like protein, regulates the formation of lateral flagella in V. parahaemolyticus TH3996,which is a strain that expresses TRH, a major virulence protein (Park et al., 2005). In addition, LonS, OpaR , and SwrT are involved in the formation of lateral flagella (Stewart et al., 1997; Enos-Berlage et al., 2005; Jaques and McCarter, 2006). Flagella biofilm formation, and virulence in pathogenic bacteria (Kawagishi et al., 1996; Ottemann and Miller,1997). For example, the lateral flagella of V.parahaemolyticus are adapted for colonization on solid or mucosal surfaces and may also bind chitin(Belas and Colwell, 1982). In addition, its lateral flagella are involved in the formation of biofilm (Park et al., 2005), which is a matrix of bacterial communities on surfaces (Davey and O;toole, 2000;O;Toole et al., 2000). In V. parahaemolyticus , biofilm formation is mediated by many factors, including extracellular polysaccharides, mannose-sensitive hemagglutinin (MSHA) type 4 pili, chitin-regulated pili (ChiRP), and OpaR (Enos-Berlage et al., 2005;Shime-Hattori et al., 2006; Yildiz and Visick, 2009).However, the relationship between flagella proteins and biofilm formation is not clear and little is known about the pathogenic role of either polar or lateral flagella in V. parahaemolyticus .
As a result, we examined the phenotypic effect of single- and double-deletion mutants of the lafA and flhAB flagellum genes in this bacterium. These mutant strains exhibited significantly less biofilm formation, cell adhesion, and colonization of the small intestine of suckling mice compared to the wild-type.
mobilization. E. coli and V. parahaemolyticus were cultured in Luria-Bertani (LB) medium or LB broth with 3% NaCl at 35°C or 28°C, respectively.Thiosulfate-citrate-bile salts-sucrose agar (TCBS)agar (Nissui, Tokyo, Japan) and LB broth with 3%NaCl were used for screening mutant strains and biofilm formation assays. When necessary, the media were supplemented with antibiotics: ampicillin (25 or 100 μg/mL), gentamicin (10 μg/mL), and chloramphenicol(5 μg/mL).
For motility assays, we inoculated semisolid tryptone swarm plates containing 1% Bacto-tryptone,2% NaCl, and 0.3% Bacto ™ agar (Difco, Detroit, MI,USA) with 2 μL of an overnight culture of bacteria normalized to an optical density of 1.0 at 600 nm(OD 600 ). These plates were incubated at 28°C for 12 h,and then the motility of bacteria was assessed qualitatively by examining the circular swarms formed by the growing bacterial cells.
The lafA (VPA1548, lateral flagellin gene), flhAB (VP2235 and VP2236, polar flagella assembly genes),and β-lactamase (VPA0477) deletion mutants of V.parahaemolyticus TH3996 were constructed using overlap extension-PCR, as described previously (Park et al., 2005). To construct the lafA mutant, the primers were 1548-1 (5'-GGATCCCTTGTAACTCA AAAC-3'), 1548-2 (5'-TCAAAACCACCACCATC AGCGTCCATTGCT-3'), 1548-3 (5'-AGCAATGG ACGCTGATGGTGGTGGTTTTGA-3'), and 1548-4(5'-GGATCCATGATACGGCCTTTA-3'). To construct the flhAB mutant, the primers were 2235-1 (5'-GGATCCAACTTAG CATGGATG-3'), 2235-2 (5'-AACGTTCAGCGCC AAGTTTTCTGCTTATAA-3'),2235-3 (5'-TTATAAGCAGAAAACTTGGCGCTGA ACGTT-3'), and 2235-4 (5'-CTGCAGAAATCTGC CTCTTTG-3'). To construct the β-lacta-mase mutant,the primers were 0477-1 (5'-CAAACTTGGATCC ATTGCGCA-3'), 0477-2 (5'-TAGGGCGTTATCT TCTTTGCCGCTGTCCAT-3'), 0477-3 (5'-ATGGA CAGCGGCAAAGAAGATAACGCCCTA-3'), and 0477-4 (5'-CATTTGAGACTGCAGGTAAGA-3').
The final PCR products were cloned into the pT7Blue T-Vector (Novagen, Madison, WI, USA)and then restriction-digested. Restriction fragments were subsequently cloned into the pYAK1 suicide vector (Park et al., 2005). After introducing the resulting plasmids into E. coli SM10λ pir (Miller and Mekalanos, 1988), the transformed bacteria were conjugated with V. parahaemolyticus TH3996.Finally, the deletion mutants were screened on TCBS agar plates containing 5 μg/mL chloramphenicol and then selected on LB plates supplemented with 10%sucrose.
Whole-cell lysates of bacteria (10 6 CFU) were resolved on 10% sodium dodecyl sulfate-polyacrylamide gel electrophoresis gels. Afterward, the proteins were transferred to an Immobilon-P transfer membrane (Millipore, Bedford, MA, USA). The membrane was blocked with 5% skim milk in Trisbuffered saline (20 mM Tris, 137 mM NaCl, pH 7.6)containing 0.1% Tween 20 and then probed with antiflagellin antibody (1:3,000 dilution) for 30 min at room temperature. The secondary antibody was a horseradish peroxidase-conjugated anti-rabbit immunoglobulin(1:5,000 dilution) for 30 min at room temperature (Amersham, Piscataway, NJ, USA).Finally, the blots were visualized by using the enhanced chemiluminescence Western blotting kit(Amersham).
HeLa cells (2×10 5 ) were grown in Dulbecco’s modified Eagle’s medium (Sigma, St. Louis, MO,USA) supplemented with 10% fetal bovine serum(Sigma) in 12-well plates in a humidified atmosphere with 5% CO 2 at 37°C overnight. In addition, overnight cultures of V. parahaemolyticus strains were diluted 1:100 in fresh LB broth containing 3% NaCl and grown at 37°C to the late log phase. Subsequently,the cells were harvested by centrifugation, resuspended in phosphate-buffered saline (PBS, pH 7.2)and then used to infect HeLa cells at a multiplicity of infection of 10. After 1.5 h, non-adherent bacteria were removed by washing the plates with PBS. The adherent bacteria were then recovered by treatment with 0.2% Triton X-100 (Sigma) for 5 min at room temperature and then plated on LB agar containing 3% NaCl. The percentage adherence was calculated by dividing the adherence of the tested strains by that of the wild-type strain.
Overnight cultures of bacteria were inoculated at a 1:100 dilution into LB broth supplemented with 3%NaCl in borosilicate glass tubes and incubated for 24 h at 28°C. After rinsing the tubes with distilled water to remove non-adherent cells, they were filled with 1.0-mL of 0.2% crystal violet solution (Junsei Chemical Co., Ltd., Tokyo, Japan), incubated for 15 min, and then rinsed vigorously with distilled water.Subsequently, the dye was removed from the cells with 1.0 mL of dimethyl sulfoxide, and biofilm formation was quantified by measuring the optical density of this solution at 570 nm. All assays were performed in triplicate.
We used the suckling mouse colonization assay of Gardel and Mekalanos (1996) with slight modifications.Briefly, 1:1 mixtures of mutant and parental strains of V. parahaemolyticus TH3996 (about 3×10 5 total cells) were administered intragastrically to CD-1 suckling mice (5-6 days old). After 24 h, the small intestine was homogenized, and then adequately diluted samples were plated on TCBS agar with or without 25 μg/mL ampicillin. The competitive index was calculated as the ratio of mutant/parental strains that were recovered from the small intestine. The mean competitive index was the average of four assays, each with at least five mice.
The lafA, flhAB, and double-deletion mutant strains were confirmed by PCR and Southern blotting, and their in vitro growth curves were indistinguishable from that of the wild-type strain (data not shown).Furthermore, Western blotting showed that polar flagellin was expressed in the wild-type strain and lafA deletion mutant strain but not in the flhAB deletion mutant or double-mutant strains ( Fig. 1 ).Similarly, lateral flagellin was expressed in the wildtype strain and flhAB deletion mutant strain but not in the lafA deletion mutant or double-mutant strains ( Fig.1 ). These results indicate successful construction of three types of deletion mutant strains.
Western blot analysis of whole-cell lysates of wild-type and flagella gene mutant strains of Vibrio parahaemolyticus. Lane 1 wild-type strain; lane 2lafA deletion mutant strain; lane 3 flhAB deletion mutant strain; lane 4 lafA/flhAB double mutant strain.
Motility assay of wild-type and flagella genedeletion mutant strains of Vibrio parahaemolyticus.A wild-type strain; B lafA deletion mutant strain; CflhAB deletion mutant strain; D lafA/flhAB doublemutant strain.
that of the wild-type ( Fig. 2A - 2C ). The small amount of motility in the lafA deletion mutant was most likely due to the residual activity of polar flagella.The double-mutant strain was nonmotile ( Fig. 2D ). Consequently, these results coincided with the Western blot analysis shown in Fig. 1 .
Ability of wild-type (WT) and flagella gene deletion mutant strains of Vibrio parahaemolyticus to form biofilms. Results are expressed as the mean of three independent experiments. Error bars represent SDs.
strain. Not surprisingly, the double mutant exhibited the most severely impaired biofilm formation.
In the adherence assays, the lafA, flhAB , and double-mutant strains showed 40%, 45%, and 60%,respectively, less adherence to HeLa cells than the wild-type strain ( Fig. 4 ). Together, these results demonstrated that both polar and lateral flagella of V.parahaemolyticus are critical for biofilm formation and cell adhesion.
Adherence of wild-type (WT) and flagella gene deletion mutant strains of V. parahaemolyticus to HeLa cells. Results are expressed as the ratio of the adherence of the tested strains to that of the wild-type strain. Error bars represent SDs.
The lafA, flhAB , and double-mutant strains exhibited 49%, and 5.6 and 6.7 times lower colonization,respectively, in the competition assay than the wild-type ( Table 2 ). These results indicated that the ability of V. parahaemolyticus to colonize the small intestine of suckling mice depends more on polar than lateral flagella.
Infant mouse colonization assay of dual flagella-related gene deletion mutants*TThe competition index is given as the ratio of output mutant to wild type (recovered from the intestine)divided by the ratio of input mutant to wild type(inoculated into a mouse). Thus, if a mutant has no colonization defect, we expect a competitive index close to 1.
Infant mouse colonization assay of dual flagella-related gene deletion mutants	*TThe competition index is given as the ratio of output mutant to wild type (recovered from the intestine)divided by the ratio of input mutant to wild type(inoculated into a mouse). Thus, if a mutant has no colonization defect, we expect a competitive index close to 1.
Although many studies have characterized flagellum genes and proteins of the dual flagella system of V. parahaemolyticus , few have investigated their pathogenic role. Moreover, the role of the polar flagella is less clear than that of the lateral flagella. In this study, we constructed three flagellum gene deletion mutant strains of V. parahaemolyticus and determined their effects on biofilm formation, cell adhesion, and colonization of the small intestine of suckling mice. Our results were consistent with previous studies, which demonstrated that lateral and polar flagella are associated with cell adhesion and colonization (Belas and Colwell, 1982) as well as biofilm formation (Enos-Berlage et al., 2005; Park et al., 2005). Similar studies on two other Vibrio spp.,namely V. vulnificus and V. cholerae , also suggested that the loss of flagellum genes usually results in decreased attachment, biofilm formation, and virulence (Watnick et al., 2001; Lee et al., 2004).However, unlike V. parahaemolyticus , neither V.vulnificus nor V. cholerae possesses lateral flagella.In the adherence and biofilm formation assays in this study, the flagellum gene deletion mutant strains of V.parahaemolyticus exhibited significantly less adherence to HeLa cells and biofilm formation than the wild-type. Therefore, our data suggest that lafA and flhAB are positively regulated with other genes that are related to cell adhesion and biofilm formation,such as those that control the expression of pili, outer membrane proteins, capsular polysaccharides, and exopolysaccharides. Furthermore, in the competition assay in suckling mice, both the flhAB and doublemutant strains showed a severe colonization defect, however, the lafA mutant strain did not exhibit significantly reduced colonization. These results suggest that polar flagella are more important than lateral flagella for colonization. Since lateral flagella of wild-type V. parahaemolyticus are extremely unlikely to form in liquid environments, we hypothesize that they cannot be formed in the small intestine of mice. Therefore, further study is needed to elucidate the expression pattern of lateral flagella in V. parahaemolyticus .
In conclusion, this study showed that both the lateral and polar flagella of V. parahaemolyticus are involved in biofilm formation, cell adhesion, and colonization of the small intestine in suckling mice.This study has important implications for further research into the pathogenesis of V. parahaemolyticus .
This research was supported by Basic Science Research Program through the National Research Foundation of Korea (NRF) funded by the Ministry of Education, Science and Technology (2010-0003640) and by the Research Fund of the Kunsan National University of Korea.
 HG Lee , BG Jeong , and KS Park , “Role of Dual Flagella in the Pathogenesis of Vibrio parahaemolyticus”, Fisheries and aquatic sciences, vol. 2, no. 2, Jun 2011.

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