flrA, flrB and flrC regulate adhesion by controlling the expression of critical virulence genes in Vibrio alginolyticus

Adhesion is an important virulence trait of Vibrio alginolyticus. Bacterial adhesion is influenced by environmental conditions; however, the molecular mechanism underlying this effect remains unknown. The expression levels of flrA, flrB and flrC were significantly downregulated in adhesion-deficient V. alginolyticus strains cultured under Cu2+, Pb2+, Hg2+ and low-pH stresses. Silencing these genes led to deficiencies in adhesion, motility, flagellar assembly, biofilm formation and exopolysaccharide (EPS) production. The expression levels of fliA, flgH, fliS, fliD, cheR, cheV and V12G01_22158 (Gene ID) were significantly downregulated in all of the RNAi groups, whereas the expression levels of toxT, ctxB, acfA, hlyA and tlh were upregulated in flrA- and flrC-silenced groups. These genes play a key role in the virulence mechanisms of most pathogenic Vibrio species. Furthermore, the expression of flrA, flrB and flrC was significantly influenced by temperature, salinity, starvation and pH. These results indicate that (1) flrA, flrB and flrC are important for V. alginolyticus adhesion; (2) flrA, flrB and flrC significantly influence bacterial adhesion, motility, biofilm formation and EPS production by controlling expression of key genes involved in those phenotypes; and (3) flrA, flrB and flrC regulate adhesion in the natural environment with different temperatures, pH levels, salinities and starvation time.


INTRODUCTION
Vibrio alginolyticus is an important opportunistic pathogen and causes vibriosis, one of the most prevalent diseases in maricultured animals and seafood consumers. 1 The large yellow croaker (Pseudosciaena crocea) is one of the most economically important maricultured fish species in southeast China. 2 V. alginolyticus readily causes vibriosis in cultured P. crocea, which results in severe economic losses in the warm-water season. 3 Bacterial adhesion to host surfaces is one of the initial steps in the infection process. 4,5 Host mucus is abundantly found on the surface of the skin, gills and gut lining; therefore, it is the first site of interaction between the pathogen and its host. 6 Thus, research into adhesion of pathogenic bacteria to host mucus has gained much interest 7,8 and the genes involved in bacterial adhesion are starting to be explored. 9,10 However, to our knowledge, the studies on the genetic regulation of adhesion in pathogenic bacteria conducted thus far are limited, and the genetic regulatory network is still largely unknown.
Bacterial adhesion of pathogenic V. alginolyticus to the mucus of P. crocea has been studied by our laboratory for several years. The characteristics of V. alginolyticus adhesion were found to correlate with its epidemiologic characteristics, 11,12 and bacterial adhesion was found to be influenced by environmental factors such as temperature, pH and salinity, among others. 13 To explore the mechanisms by which environmental factors influence bacterial adhesion, pathogenic V. alginolyticus was subcultured under nine different stress conditions. Of these, Cu 2+ , Pb 2+ , Hg 2+ and low pH were found to reduce the adherence of V. alginolyticus, whereas high pH, low or high salinity, and low or high temperature did not significantly affect adhesion. 14 Next, the adhesion-attenuated culture and a control culture were subjected to RNA-seq. 14 The RNA-seq results indicated a role for the flagellar assembly genes and three noncoding RNAs, and these were further studied to determine their role in bacterial adhesion. 3, 15 The flagellum has been shown to be involved in bacterial adhesion and invasion of host cells, as it is used in motility, chemotaxis and as an adhesin. 16 The synthesis and assembly of the flagellum is a tightly regulated process. 17 flrA, rpoN, flrB and flrC are part of a twocomponent system 18 that is considered a key prerequisite for bacterial pathogenesis. 19 The histone-like nucleoid-structuring protein and the general stress-response regulator RpoS could enhance the transcription of flrA and rpoN. 20 Both of FlrA and RpoN-bound RNA polymerase could activate the transcription of class II flagellar genes. 21 The flrA transcription start is 68 bp upstream from the flrA translation start site, and DNA sequence upstream of the transcription start contains a σ 70 promoter sequence (TTGACA-N14-TGGCACTTT). 22 FlrA could directly bind to the flrBC promoter. The binding site is 73-53 bp from the transcription start site (consisted of an inverted repeat sequence of ATTG(A/G)C), which is 24 bp upstream of the translation start site of the flrBC operon. 23 FlrB and FlrC could activate the transcription of class III genes. 21 flrA, flrB and flrC were first identified in V. cholerae and shown to be required for flagellar synthesis. 21 Since then, only a few related studies were performed and mainly focused on the role of flrA, flrB and flrC in flagellar synthesis. 17,24 However, the role they and their downstream genes have in the virulence mechanisms of most pathogens is poorly understood and remains to be elucidated.
The results of RNA-seq by our laboratory showed that flrA, flrB and flrC were significantly downregulated under several stress conditions (Cu 2+ , Pb 2+ , Hg 2+ and low pH). As V. alginolyticus adhesion was also significantly inhibited by these four stress conditions, these genes were hypothesized to have a role in bacterial adhesion. Here, we examine the genes that contribute to adhesion of pathogenic V. alginolyticus. The purpose of our study was to investigate (i) the relationship between flrA, flrB, flrC and V. alginolyticus adhesion; (ii) how these genes affect adhesion; and (iii) whether these genes participate in the regulation of adhesion in natural conditions.

MATERIALS AND METHODS
Bacterial strain and culture conditions Pathogenic V. alginolyticus (ND-01) was isolated from a spontaneously infected P. crocea and previously identified as pathogenic by subsequent artificial infection. 25 Bacteria were stored in physiological saline with 10% glycerol at − 80°C. Bacteria were grown in LB 20 medium (Luria-Bertani medium plus 2% NaCl) 26 with shaking at 220 rpm.
RNA sequencing (RNA-Seq) results were confirmed by quantitative reverse transcriptase real-time polymerase chain reaction (qRT-PCR). V. alginolyticus was stressed with 50 mg/L Cu 2+ , 100 mg/L Pb 2+ , 50 mg/L Hg 2+ or low pH (HCl was used to lower the pH to 5). As a control, V. alginolyticus was also incubated under normal conditions (LB 20 broth with 2% NaCl, pH = 7). Each treatment consisted of six independent biological replicates (three technical replicates within each).
To investigate the effects of different temperatures, V. alginolyticus was cultured in LB 20 broth (supplemented with 2% NaCl, pH = 7) at 41C, 151C, 281C, 371C and 44°C. To investigate the effects of different pH levels, V. alginolyticus was cultured in LB 20 broth (supplemented with 2% NaCl) adjusted to a pH of 5, 6, 7, 8 or 9. 11 To investigate the effects of different salinities, V. alginolyticus was cultured in LB 20 broth (pH = 7) with 0.8%, 1.5%, 2.5%, 3.5% or 4.5% NaCl. 11 To investigate the effects of starvation, V. alginolyticus was cultured in normal phosphate-buffered saline (PBS) at 28°C for one, three, five and seven days. 27 Each treatment consisted of six independent biological replicates (three technical replicates within each). After harvesting and re-suspending, RNA was extracted from the bacteria, and reverse transcription and qRT-PCR were performed.
Functional classification and enrichment analysis of differentially expressed genes To annotate identified differentially expressed genes (DEGs), the Blast2GO program was used to obtain Gene Ontology (GO) annotations for each unigene. After obtaining the GO annotation of each unigene, the WEGO software (BGI, Shenzhen, China) was used to determine GO functional categories of all unigenes and to illustrate the species layout of unigene functions in a macroscopic view. The Bonferroni correction was used to calculate the P-value. Adjusted P ⩽ 0.05 was used as a threshold. GO terms satisfying this criterion were defined as notably enriched GO terms from the DEGs.
Kyoto encyclopedia of genes and genomes (KEGG) pathway annotations were obtained using the Blastall software (NCBI, Bethesda, MD, USA; http://www.ncbi.nlm.nih.gov/BLAST/) and the KEGG (http://www.genome.jp/kegg/) database. Q-values were defined as the false discovery rate analog of the P-value. Pathways with Q ⩽ 0.05 were deemed significantly enriched in DEGs.

Transient gene silencing
Negative control short interfering RNA (siRNA) and treatment siRNA sequences (targeting at 136 bp-155 bp downstream from the flrA translation start site, 728 bp-747 bp downstream from the flrB translation start site and 935 bp-954 bp downstream from the flrC translation start site) were chemically synthesized by GenePharma Co. Ltd (Shanghai, China) and are listed in Supplementary Table S1.
Electrotransformation of bacteria was performed following the method of Lancashire et al. 28 Overnight cultures of V. alginolyticus were inoculated into fresh LB 20 broth (1:100 v/v) and incubated until the OD 600 reached 0.3-0.5. Bacterial cells were harvested by centrifugation at 4000 g for 10 min at 4°C, thoroughly washed twice with ice-cold sterile water at 4°C and subsequently washed once in ice-cold 10% washing buffer (10% redistilled glycerol, 90% sterile water, v/v). Finally, the competent cells were re-suspended in 1 mL ice-cold 10% glycerol and stored at − 80°C for a short time.
V. alginolyticus-competent cells were electroporated using a Bio-Rad MicroPulser (Bio-Rad Laboratories Inc., Hercules, CA, USA) following the method of Huang et al. 15 Two microliters of 20 μM siRNA was vigorously mixed into 100 μL of electrocompetent cells. After incubating on ice for 30 min, the mixture of cells/siRNA was transferred into an electroporation cuvette and electroporated at 1.8 kV for 6 ms. Then, 900 μL of room temperature LB 20 medium was immediately added, and the cells were shaken for 1 h, 6 h, 12 h and 24 h at 28°C for RNA extraction and qRT-PCR.

Stable gene silencing
The stable gene-silencing assay for V. alginolyticus was implemented based on Darsigny et al. 29 and Choi and Schweizer. 30 Overnight cultures of V. alginolyticus were collected by centrifugation and treated as described in the transient gene-silencing section. Three short hairpin RNA sequences targeting at 136 bp-155 bp downstream from the flrA translation start site, 728 bp-747 bp downstream from the flrB translation start site and 935 bp-954 bp downstream from the flrC translation start site were designed by Shanghai Generay Biotech Co., Ltd (Shanghai, China; Supplementary Table S2). The annealed oligonucleotides were ligated with pACYC184 vectors, which were harvested from BamHI and SphI double digestion via T4 DNA ligase (TaKaRa, Kusatsu, Japan) according to the manufacturer's recommendations. Competent E. coli SM10 cells were transformed with the recombinant pACYC184 vectors via heat-shock and then transferred by conjugation from E. coli SM10 to V. alginolyticus. The empty plasmid pACYC184 was also transferred into cells and used as the control strain. The stable silenced clones were screened using LB 20 medium containing chloramphenicol (34 μg/mL).

Mucus preparation
P. crocea care and use were conducted in strict accordance with the recommendations in the 'Guide for the Care and Use of Laboratory Animals' set by the National Institutes of Health. The protocol was approved by the Animal Ethics Committee of Xiamen University (Acceptance NO XMULAC20120030).
Healthy P. crocea were obtained from marine cultured cages in the city of Ningde (Fujian, China) and were used for mucus preparation flrA, flrB and flrC regulate bacterial adhesion G Luo et al as previously described. 31 After careful washing in PBS (0.01 mol/L pH 7.2), the skin mucus was collected by gently scraping the skin surface using a soft rubber spatula and was then homogenized in PBS. The homogenate was centrifuged twice (20 000g, 4°C, 30 min), and the supernatant was filtered through 0.45-μM and 0.22-μM pore-size filters. Finally, PBS was added to each mucus sample to obtain a final concentration of 1 mg protein/mL, as determined by a Bradford assay. 32 In vitro adhesion assay The bacterial adhesion assay was carried out as described in our previous study. 33 P. crocea mucus (50 μL) was evenly coated onto a 22-mm 2 area of a glass slide area and fixed by methanol for 20 min. One milliliter of a bacterial suspension (10 8 colony-forming unit/mL) was spotted onto a mucus-coated glass slide. Then, the glass slides were placed in a humidified chamber, incubated at 25°C for 2 h and then washed five times in PBS. Finally, the bacteria were fixed with 4% methanol for 30 min, stained with crystal violet for 3 min and counted under a microscope (×1000). Three independent biological replicates (three technical replicates within each) were performed per group, and 20 random fields within each technical replicate were chosen to count. For the transient silencing, wild V. alginolyticus containing negative control siRNA (non-targeting) was used as a control group. For the stable silencing, wild V. alginolyticus containing empty plasmid pACYC184 was used as a control group.

RNA extraction and reverse transcription
Total bacterial RNA was extracted with TRIzol reagent (Invitrogen, Carlsbad, CA, USA) following the manufacturer's instructions. First-strand complimentary DNA (cDNA) synthesis was performed with a RevertAid Mu-MLV cDNA Synthesis Kit (TransGen Biotech) following the manufacturer's instructions.

qRT-PCR
The expression levels of genes were determined by qRT-PCR using QuantStudio 6 Flex (Life Technologies, Grand Island, NY, USA). Expression levels were normalized to 16S rRNA and then calculated using the 2 − ΔΔCt method; primer sequences are listed in Supplementary Table S3.
Transmission electron microscope observation Wild-type and stably silenced V. alginolyticus were cultured in LB 20 broth at 28°C for 16 h. Then, the culture was mounted onto formvarcoated copper grids by floating the grids on drops of sample for 1 min. The grids were washed three times in sterile deionized water to remove the medium. The cells were negatively stained by floating the grids on a drop of 1% phosphotungstic acid and then viewed using a transmission electron microscope (Philips, Tecnai F20, Amsterdam, Holland). More than 20 fields of view were randomly selected in each group. The length and diameter of flagella were measured with the Osiris 4.0 software (Geneva, Switzerland) from images (n = 6 cells per condition).

Soft agar plate motility assay
The soft agar method was used to assay the motility of V. alginolyticus strains. Briefly, fresh overnight cultures were diluted to an OD 660 of 0.03 in LB 20 . The cell suspension (1 μL/drop) was dropped onto the center of semisolid agar plates (LB 20 broth+0.5% agar) and the plates were allowed to incubate for 20 h at 28°C before measuring the colony diameters; three independent biological replicates (three technical replicates within each) were performed per group.

Biofilm assay
The biofilm assay for V. alginolyticus was implemented based on Lee et al. 34 V. alginolyticus strains were grown (overnight, 28°C) in LB 20 and then adjusted to the same OD 600 . Bacterial culture (50 μL) was added to 150 μL of LB 20 per well of a 96-well plate and then incubated at 28°C for 24 h. Wells were rinsed with sterile PBS, incubated (30 min) with 200 μL crystal violet (1%), washed with sterile PBS and air-dried. The stained biofilm was solubilized with 200 μL 33% acetic acid and then quantitated by measuring OD 570 ; three independent biological replicates (three technical replicates within each) were performed per group.

Quantification of exopolysaccharide
Purification and quantification of exopolysaccharide (EPS) were performed using a slight modification of the methods of Acosta et al. 35 and Kimmel et al., 36 respectively. Overnight cultures of V. alginolyticus were boiled (10 min) and centrifuged (12 000 rpm, 20 min) to remove cells. Trichloroacetic acid (10% final concentration) was added to precipitate proteins and polypeptides. After centrifugation, a filter membrane (0.45 µM) was used to filter the supernatant. Ice-cold ethanol (1 volume) was added to the supernatant fluid, and the coarse EPS was precipitated. After centrifugation, it was re-suspended in sterile distilled water (1/10th the original volume) and dialyzed in dialysis tubing. Phenol (0.3 mL, 6%) was added to the dialyzed EPS (0.5 mL), and then 1.5 mL concentrated sulfuric acid was quickly added and the mixture was shaken. This solution was heated for 15 min in a 100°C water bath, cooled in cold water and finally quantitated by measuring OD 490 ; three independent biological replicates (three technical replicates within each) were performed per group.

Hemolysis assay
Hemolysis assays were carried out as described by Tsou and Zhu. 37 Rabbit blood (Ping Rui Biotechnology Co., Ltd, Beijing, China) was prepared by washing three times with PBS. Washed rabbit blood (5 µL) was added to 245 µL of culture supernatants and incubated at 37°C for 1 h under the relatively mild shaking conditions. After incubation, samples were centrifuged, and the released hemoglobin was measured by OD 540 . The percentage of total hemolysis was calculated by comparing the OD 540 of the samples with positive (100% lysis by 1% Triton X-100) and negative controls.

Data processing
The data are presented as the mean ± SD. Statistical analysis was performed by one-way analysis of variance with Dunnett's test using the SPSS 13.0 software (Chicago, IL, USA). P-valueo0.05 were considered statistically significant.

RNA-seq screening and validation for DEGs
The RNA-seq results for V. alginolyticus cultured under Cu 2+ , Pb 2+ , Hg 2+ and low-pH conditions (V. alginolyticus cultured under normal condition was used as a control group) have been deposited in the NCBI Sequence Read Archive (Accession NO SRP049226). RNA-seq and DEG analysis finally yielded 1637, 1085, 846 and 1791 DEGs in the Cu-, Pb-, Hg-and low-pH-treated groups compared with the control group, respectively. Analysis of GO categories showed that the functional distribution of the DEGs from each stressed group was similar. In the libraries, most of the corresponding biological process genes were involved in cellular processes, metabolic processes, establishment of localization and localization. Most of the cellular flrA, flrB and flrC regulate bacterial adhesion G Luo et al component genes encoded proteins associated with cell, cell part, membrane and membrane part; moreover, most of the molecular function genes were associated with binding and catalytic activity. Using KEGG, DEGs were assigned to 164 KEGG pathways. Those pathways with the greatest representation by DEGs were 'ABC transporter system', 'Two-component system', 'Glyoxylate and dicarboxylate metabolism' and 'Flagellar assembly'. These annotations provide a substantial resource for investigating specific processes, functions and pathways during bacteria adherence. Among the 164 KEGG pathways, some pathways are known to be closely related to adhesion, for example, 'Two-component system', 'Bacterial chemotaxis' and 'Flagellar assembly'. In the present research, the Two-component system was selected for further research. GO and KEGG analyses revealed that there are 67 DEGs involved in Two-component systems. Among the DEGs, FlrA, FlrB and FlrC were generally significantly downregulated in all four of the stressed groups (Table 1).

Effects of transient gene silencing
The mRNA levels of the three target genes in V. alginolyticus were determined at 1, 6, 12 and 24 h after electrotransformation. Treatment of V. alginolyticus with siRNA ( Figure 2A) induced significant gene silencing (Po0.05) in V. alginolyticus show at 1-6 h; however, the silencing effect of each siRNA was not significant at any of the time points after 6 h. The decline in mRNA levels of each target gene revealed that the siRNA worked.
Thus, the in vitro assay for V. alginolyticus adhesion was performed under normal and RNAi conditions to further verify the silencing effect of siRNA at 2 h after electrotransformation. The number of adherent cells was counted. In the control group,~1248 ± 96 cells/view adhered to the glass. In contrast, in the flrA-, flrBand flrC-RNAi groups,~277 ± 40, 207 ± 12 and 463 ± 38 cells/view adhered to the glass, respectively ( Figure 2B).
These data show that the number of adherent cells was significantly lower in the RNAi groups than in the control group. The results of this   adhesion assay indicate that RNAi significantly impairs V. alginolyticus adhesion to P. crocea mucus.

Effects of stable gene silencing
The mRNA levels of flrA, flrB and flrC were significantly lower (by 12.86-fold, 3.71-fold and 5.03-fold, respectively) in the stably silenced V. alginolyticus ( Figure 3A). These data indicate that the stable gene silencing was reliable in this study. The stably silenced V. alginolyticus exhibited a significant decrease in adhesion. In the control V. alginolyticus,~1435 ± 122 cells/view adhered to the glass. However, in the flrA-, flrBand flrC-RNAi V. alginolyticus,~263 ± 15, 480 ± 36 and 367 ± 18 cells/view adhered to the glass, respectively ( Figure 3B). The adhesion assay results indicate that stable gene silencing significantly impairs V. alginolyticus adhesion to P. crocea mucus.
The expression levels of 12 important downstream virulence genes in the stably silenced V. alginolyticus are shown in Table 2. Compared with the control group (strain with the empty plasmid pACYC184), the expression levels of fliA, flgH, fliS, fliD, cheR, cheV and V12G01_22158 exhibited significant downregulation in all three of the RNAi groups, whereas the expression levels of toxT, ctxB, acfA, hlyA and tlh exhibited upregulation in the flrAand flrC-RNAi groups. These data indicate that the expression levels of the majority of these virulence genes were affected by RNAi of flrA, flrB and flrC. For the upregulated genes, flrA-RNAi exhibited a more powerful effect than flrB-RNAi and flrC-RNAi. Furthermore, the expression of toxT, ctxB, acfA, hlyA and tlh was unchanged in the flrB stably silenced strain compared with the control. For the downregulated genes, flrB-RNAi exhibited a more powerful effect than flrA-RNAi and flrC-RNAi; however, the decrease in fliD transcription was most obvious in the flrA stably silenced strain.
The flagella of stably silenced clones were observed ( Figure 4). The data revealed that flagella were present on the control and flrA-RNAi strains, whereas the flagella of the flrA-RNAi strain were significantly thinner and shorter compared with the control (Po0.01). However, no flagella could be observed on the flrB-RNAi and flrC-RNAi strains. Figure 5 shows different levels of V. alginolyticus motility on soft agar plates. The results indicated that flrA-RNAi, flrB-RNAi and flrC-RNAi resulted in reduced motility of V. alginolyticus, whereas flrB-RNAi and flrC-RNAi were more effective than flrA-RNAi.
Biofilm formation of stably silenced clones was measured at OD 570 ( Figure 6). The data showed that the ability to form biofilms was significantly decreased in flrA-RNAi, flrB-RNAi and flrC-RNAi compared to the wild-type strain, whereas flrB-RNAi was more effective than flrA-RNAi and flrC-RNAi (Po0.05). Figure 7 shows the production of EPS in different V. alginolyticus strains. The results revealed that EPS production of flrA-RNAi, flrB-RNAi and flrC-RNAi was significantly lower than the control, whereas the EPS production of flrB-RNAi was the lowest of the three stably silenced strains (Po0.05).
The hemolytic activity of V. alginolyticus strains during stress conditions of Cu 2+ , Pb 2+ , Hg 2+ and low pH, and during stable gene silencing has been detected ( Figure 8). The V. alginolyticus strains under stress conditions of Cu 2+ , Pb 2+ , Hg 2+ and low pH showed increased levels of a hemolytic activity against rabbit erythrocytes compared with the V. alginolyticus strains under normal condition ( Figure 8A). The Figure 8B shows that hemolytic activity was significantly increased in flrA-RNAi and flrC-RNAi compared with the wild-type strain, and flrA-RNAi was more effective than flrC-RNAi, whereas hemolytic activity was not significantly increased in flrB-RNAi compared with the wild-type strain.    Figure 9A). flrA, flrB and flrC expression levels were the lowest at 1.5% salinity; however, they later rose with increasing salinity ( Figure 9B). Increasing starvation time also tended to reduce the expression levels of flrA, flrB and flrC ( Figure 10A). Expression of flrA, flrB and flrC was significantly affected by pH, and the highest expression levels of all the three genes occurred at pH 7 ( Figure 10B).
These data indicate that flrA, flrB and flrC may participate in regulation of adhesion in the natural environment.

DISCUSSION
Bacterial adhesion is ultimately regulated by genes. 38 Several adhesionrelated genes have been identified in V. alginolyticus, 3 Pseudomonas putida, 39 P. aeruginosa, 39 Candida albicans, 40 E. coli 41 and Erysipelothrix rhusiopathiae. 42 However, more details about the mechanism have not been found.
In our previous research, 14 V. alginolyticus adhesion was significantly reduced by Cu 2+ , Pb 2+ , Hg 2+ and low pH. What's more, flrA, flrB and flrC were generally downregulated under the four stress conditions tested. The flagellum has been shown to be involved in bacterial adhesion, 16 whereas flrA, flrB and flrC are required for the synthesis and assembly of the flagellum. 21 We do not think this is a coincidence. Therefore, we hypothesized a connection between them. In the present study, RNAi-mediated silencing of these three genes reduced bacterial adhesion. These results demonstrate that flrA, flrB and flrC have a key role in V. alginolyticus adhesion.
Bacterial adhesion has been demonstrated to be affected by bacterial motility 19 and chemotaxis. 16 Indeed, bacterial motion and chemotaxis rely on the synthesis and assembly of the flagellum. 43 Transcription of      (Table 2). Nevertheless, it is hard to draw a common conclusion for the regulatory mechanism from the presented experimental results. Interestingly, the downregulation of fliA, flgH, fliS, cheR and cheV in the flrB-RNAi strain was more distinct than in the flrA-RNAi and flrC-RNAi strains. We also showed that the flrB-RNAi has more significant effects on flagella assembly and motility than the flrA- The bacterial adhesion process was also directly mediated by adhesins, 16,46 which are widely distributed on the bacterial surface. 47 V12G01_22158 is a gene that has recently been identified in pathogenic V. alginolyticus and encodes a GGDEF protein 48 whose domain DGCs catalyze the conversion of two guanosine triphosphate into bis-(3′-5′)-cyclic dimeric guanosine monophosphate, which generally has an essential role as a ubiquitous second messenger in regulating motility, virulence, biofilm formation (associated with adhesins) 49 and EPS (an adhesin) biogenesis. 50 These results indicate that V12G01_22158 may be an important pathogenic gene in V. alginolyticus. Our data show that the expression of V12G01_22158 was significantly downregulated in every stably silenced V. alginolyticus strains (Table 2), and the three stably silenced strains had reduced Genes acfA, ctxB, hlyA and tlh have a pivotal role in the colonization and pathogenesis of Vibrio. The hlyA and tlh are hemolysin genes. 45 toxT activates transcription of acfA and ctxB. 51 It has been shown that many virulence genes are more highly expressed in flagellar regulatory mutants and can enhance V. cholerae pathogenesis. 45 In this study, flrA-RNAi resulted in significant upregulation of toxT, acfA, ctxB, hlyA and tlh, which led to significant increase in hemolytic activity. flrB-RNAi exhibited no significant effect on the expression of these five genes and hemolytic activity. flrC-RNAi resulted in significant upregulation of toxT, ctxB and tlh, which led to significant increase in hemolytic activity. Enhanced hemolytic activity was also observed for the V. alginolyticus strains under stress conditions of Cu 2+ , Pb 2+ , Hg 2+ and low pH, whereas flrA and flrC were downregulated by these conditions. Taken together, these results indicated that (i) transcriptions of acfA, ctxB, hlyA, tlh and toxT were negatively regulated by flrA, and then the hemolytic activity was repressed by flrA through hlyA and tlh; (ii) transcriptions of ctxB, tlh and toxT were negatively regulated by flrC, and then the hemolytic activity was repressed by flrC through tlh; (iii) the increase in acfA and ctxB expression is most likely because of the upregulation of toxT, which directly binds and activates acfA and ctxB. 45 Our results suggested that expression of the virulent genes toxT, ctxB and tlh was regulated by flrA and flrC, that the virulence genes acfA and hlyA were regulated by flrA, and that fliA, flgH, fliS, fliD, cheR, cheV and V12G01_22158 were regulated by flrA, flrB and flrC. flrA, flrB and flrC therefore have a significant signaling role in the pathogenicity of flagellation, motility, chemotaxis, adhesion, colonization and cytotoxicity. Moreover, flrB-RNAi led to maximum inhibition of genes associated with flagellation, motility, chemotaxis and adhesins, which translated to significant inhibition of adhesion; yet, flrB-RNAi did not increase the expression of genes associated with colonization or cytotoxicity. Therefore, flrB may be the most important gene among flrA, flrB and flrC from the perspective of disease prevention and treatment.
Many pathogenic bacteria can induce an adaptable response to environmental stimuli, primarily by altering gene expression. 19 For example, V. cholera rpoS mutants are sensitive to environmental conditions (including starvation, high osmolarity and oxidative stresses) when compared with the wild type. 52,53 In our present study, the expression levels of flrA, flrB and flrC were found to be sensitive to different temperatures, changes in pH, changes in salinities and increased starvation time (Figures 9 and 10). Our previous research showed that V. alginolyticus adhesion was remarkably influenced by those environmental factors. 11 These results suggested that the changes in expression of flrA, flrB and flrC may be an important factor influencing adhesion under those environmental conditions and further strengthened the necessity of the present study.
In conclusion, our results suggest that (i) flrA, flrB and flrC are closely associated with the process of V. alginolyticus adhesion; (ii) flrA, flrB and flrC affect adhesion by affecting motility, chemotaxis and adhesins; and (iii) flrA, flrB and flrC regulate adhesion in different natural environments. In addition, our results showed that flrA, flrB and flrC have a significant signaling role in the pathogenicity of flagellation, motility, chemotaxis, adhesion, colonization and cytotoxicity. In this paper, we present for the first time the biochemical and molecular features of the flrA, flrB and flrC in V. alginolyticus and also indicate the pathogenic implications of these genes, which provide insight into prevention and treatment of this and related diseases.