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V. cholerae El Tor C7258 was applied as the wild-type (WT) strain. Nonpolar hapR and fur single-gene mutants (ΔhapR and Δfur) and the complementary mutants ΔhapR/pBAD24-hapR (C-ΔhapR) and Δfur/pBAD24-fur (C-Δfur) were constructed as previously described[39]. The VCA0560 gene mutant (ΔVCA0560) was constructed from WT using the suicide plasmid pWM91 by the allelic exchange as previously described[40]. The coding region of the VCA0560 gene was cloned into the pBAD24 vector containing an arabinose-inducing pBAD promoter to construct the overexpression plasmid pBAD24-VCA0560[41]. The recombinant pBAD24-VCA0560 was transferred into WT to construct the VCA0560 overexpression strain WT/pBAD24-VCA0560, which produced about 3.5 times as many VCA0560 mRNA levels as that of the WT/pBAD24 strain (data not shown). The pBAD24 vector was also introduced into WT, ΔhapR, and Δfur to prepare controls. All primers used are listed in Table 1.
Target Primers (forward/reverse, 5'–3’) Construction of mutant VCA0560 GCGGGATCCGAACAGCGATCAGAGCATG/CCTCCTTTGCCAATTTTGAATTCCTGAGGTTCTACATTG CAATGTAGAACCTCAGGAATTCAAAATTGGCAAAGGAGG/GGACTAGTGCGAGTTGATGTGGGTAG GCGGGATCCGAACAGCGATCAGAGCATG/GGACTAGTGCGAGTTGATGTGGGTAG Construction of overexpressed plasmid VCA0560 GATTCTAGAATGTCTTCTAGCTTTGTTAC/GCGAAGCTTTTAGCTAGCGACTTTGACAC Luminescence assay VCA0560 GCGGAGCTCGAACAGCGATCAGAGCAT/GCGGGATCCCAGCAGCAATAGAGGAAAA EMSA VCA0560 GAACAGCGATCAGAGCAT/CAGCAGCAATAGAGGAAAA recA AAGATTGGTGTGATGTTTGGTA/CACTTCTTCGCCTTCTTTGA DNase I footprinting VCA0560 GTAAAACGACGGCCAGTCAAGCTGCAACGGCAAGTAG/CAGGAAACAGCTATGACCAGCAGCAATAG
AGGAAAAM13 FAM-GTAAAACGACGGCCAGT/CAGGAAACAGCTATGAC-HEX Table 1. Oligonucleotide primers used in this study
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Luria-Bertani (LB) broth (1% tryptone, 0.5% yeast extract, and 1% NaCl) was applied for V. cholerae cultivation[39]. Overnight bacterial cultures were diluted at 1:50 into 5 mL of fresh LB broth and grown at 30 °C with shaking at 200 rpm to an OD600 value of 1.0. The resultant cultures were diluted 1:100 into 5 mL of fresh LB broth for the third-round growth. The bacterial cells were harvested at an OD600 value of about 0.6. Whenever required, antibiotics were used in the following concentrations: 100 mg/mL ampicillin, 5 mg/mL chloramphenicol, and 0.1% arabinose.
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Colony morphology was characterized as previously described[42]. In brief, 2 μL of overnight bacterial culture was spotted onto the LB agar and then statically incubated at 30 °C for 48 h.
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CV staining was performed as previously described[42]. The third round of cultures was diluted 50-fold into 2 mL of fresh LB broth in glass tubes and then allowed to grow at 30 °C with shaking at 100 rpm for 48 h. The surface-attached cells were stained with 0.1% CV. The bound dye was dissolved with dimethylsulfoxide (DMSO), and the OD570 values were measured for each strain as the index of CV staining.
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Intracellular c-di-GMP levels were detected as previously described[13,43]. Bacterial cells were harvested at OD600 = 0.6, washed twice with ice-cold phosphate buffered solution (PBS), resuspended in 2 mL of ice-cold PBS, incubated at 100 °C for 5 min, and sonicated for 15 min (power 100%, frequency 37 kHz) in an ice-water bath. The supernatant was collected, and the pellet was resuspended in 2 mL of ice-cold PBS and re-extracted twice. The intracellular c-di-GMP levels were determined with a c-di-GMP ELISA kit (Mskbio, Beijing, China). Total protein concentration in the supernatant was also determined using a Pierce BCA Protein Assay kit (ThermoFisher Scientific, USA) in accordance with the manufacturer’s instructions. c-di-GMP concentration was expressed as pmol/mg protein.
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Swimming motility was assayed as previously described[44]. In brief, 2 μL of the third round of cell cultures were inoculated into semisolid swim plates (1% tryptone, 0.5% yeast extract, 1% NaCl, and 0.35% bacterial agar), and the diameter of the swimming areas was measured after incubation at 30 °C for about 10 h.
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A luminescence assay was performed as previously described[45]. The regulatory DNA region of VCA0560 was cloned into the pBBRlux vector harboring a promoterless luxCDABE reporter gene. The recombinant plasmid was transferred into WT and regulatory gene mutants (ΔhapR and Δfur) to measure lux activity in each strain. Luminescence was determined using an Infinite® 200 Pro NanoQuant (Tecan, Switzerland), and lux activity was calculated as light units/OD600.
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The coding regions of hapR and fur were separately cloned into the pET28a (Novagen, USA) to express His-HapR and His-Fur using Escherichia coli BL21λDE3 cells[46]. His-HapR and His-Fur were prepared as previously described [47,48]. The dialyzed proteins were concentrated to approximately 0.5 mg/mL, and their purity was analyzed by SDS-10% PAGE.
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EMSA was performed as previously described[48]. The 5ʹ-ends of the regulatory DNA region of the VCA0560 gene were labeled with [γ-32P] ATP and T4 polynucleotide kinase. DNA binding was performed in a 10 µL reaction volume containing binding buffer (1 mmol/L MgCl2, 100 μmol/L MnCl2 or 0.5 mmol/L EDTA, 0.5 mmol/L DTT, 50 mmol/L NaCl, 10 mmol/L Tris-HCl/pH 7.5, and 10 mg/mL salmon sperm DNA), labeled DNA probe, and increasing amounts of purified His-Fur or His-HapR. After incubation at room temperature for 20 min, the products were loaded onto a native 4% (w/v) polyacrylamide gel and electrophoresed in 1.0× TB or 0.5× TBE buffer for approximately 60 min at 150 V. Radioactive species were detected by autoradiography after exposure to Fuji Medical X-ray film at −20 °C. Three controls were included in each EMSA experiment: 1) a cold probe as a specific DNA competitor (the same promoter DNA region unlabeled), 2) a negative probe as a nonspecific DNA competitor (the unlabeled coding region of the 16S rRNA gene), and 3) a nonspecific protein competitor (rabbit anti-F1-protein polyclonal antibodies).
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DNase I footprinting was performed as previously described[49-51]. The results were analyzed using an ABI 3500XL DNA Genetic analyzer with GeneMarker software 2.2.
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Colony morphological characterization, CV staining, EMSA, and DNase I footprinting assays were performed at least twice with similar results. Luminescence assay and c-di-GMP quantification were performed three times, and the values were expressed as mean ± standard deviation (SD). Paired Student’s t-tests were applied to calculate statistical significance. P values less than 0.01 were considered significant.
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The growth curves of WT/pBAD24, ΔVCA0560/pBAD24, and WT/pBAD24-VCA0560 grown at 30 °C in LB broth were recorded with 1 h intervals to determine the effect of VCA0560 on the growth of V. cholerae. As shown in Figure 1, indistinguishable growth rates were observed for WT/pBAD24 and WT/pBAD24-VCA0560, indicating that VCA0560 overexpression did not affect the growth of V. cholerae. However, the ΔVCA0560/pBAD24 strain showed a slight growth defect relative to the WT/pBAD24 and WT/pBAD24-VCA0560 strains, suggesting that VCA0560 might be required for the growth of V. cholerae.
Figure 1. Growth curves of V. cholerae strains. The overnight growth cultures of WT/pBAD24, ΔVCA0560/pBAD24, and WT/pBAD24-VCA0560 were diluted at 1:100 into 20 mL of LB broth supplemented with 100 mg/mL ampicillin and 0.1% arabinose, mixed well, and then divided into a microwell plate with 300 μL in each well. V. cholerae strains were grown at 30 °C with shaking at 200 rpm, and the OD600 values were monitored at 1 h intervals. The experiment was conducted twice, with five replicates per trial for each strain.
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Colony morphological characterization and CV staining were performed to compare colony morphology and biofilm quantity among WT/pBAD24, ΔVCA0560/pBAD24, and WT/pBAD24-VCA0560. As shown in Figure 2A, WT/pBAD24 and ΔVCA0560/pBAD24 produced smooth colonies on the LB plates, and WT/pBAD24-VCA0560 formed wrinkled colonies. CV staining assay showed that WT/pBAD24-VCA0560 produced significantly more normalized CV staining than WT/pBAD24 and ΔVCA0560/pBAD24, and ΔVCA0560/pBAD24 showed similar CV staining result with WT/pBAD24 (Figure 2B). These results indicated that VCA0560 gene deletion had no regulatory activity on biofilm formation, but overexpression of the protein did induce biofilm formation by V. cholerae.
Figure 2. VCA0560 overexpression induced biofilm formation by V. cholerae. (A) Colony morphological characterization. In brief, 2 μL of overnight bacterial culture was spotted on the LB agar supplemented with 100 mg/mL ampicillin and 0.1% arabinose and then statically incubated at 30 °C for 48 h. (B) Crystal violet (CV) staining. Bacterial cells were inoculated into 2 mL of fresh LB broth supplemented with 100 mg/mL ampicillin and 0.1% arabinose in glass tubes and allowed to grow at 30 °C with shaking at 100 rpm for 48 h. The surface-attached cells were stained with 0.1% CV. The bound CV was dissolved with dimethylsulfoxide (DMSO), and the OD570 values were measured as the index of CV staining. NS represents no significant difference.
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The swimming motility assay showed that the swimming capacity of WT/pBAD24-VCA0560 was significantly inhibited relative to those of WT/pBAD24 and ΔVCA0560/pBAD24. ΔVCA0560/pBAD24 and WT/pBAD24 manifested a similar capacity for swimming motility (Figure 3). These results suggested that VCA0560 overexpression inhibited V. cholerae swimming motility.
Figure 3. Regulation of swimming motility by VCA0560 protein in V. cholerae. In brief, 2 μL of bacterial cells were inoculated into semisolid swim plates (1% tryptone, 0.5% yeast extract, 1% NaCl, and 0.35% bacterial agar) supplemented with 100 mg/mL ampicillin and 0.1% arabinose. The diameter of the swimming areas was measured after incubation at 30 °C for 10 h.
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Elevated c-di-GMP levels in bacterial cells lead to decreased motility but increased biofilm formation[5]. Thus, we further detected whether VCA0560 regulates c-di-GMP production in V. cholerae. The concentration of c-di-GMP in WT/pBAD24-VCA0560 was higher than that in WT/pBAD24 and ΔVCA0560/pBAD24. Meanwhile, ΔVCA0560/pBAD24 had similar c-di-GMP levels to WT/pBAD24 (Figure 4). These results indicated that VCA0560 mutation did not influence c-di-GMP production, but VCA0560 overexpression induced c-di-GMP synthesis in V. cholerae.
Figure 4. Intracellular c-di-GMP levels in V. cholerae strains. V. cholerae strains were cultured in LB broth supplemented with 100 mg/mL ampicillin and 0.1% arabinose at 30 °C and harvested at OD600 = 0.6. Intracellular c-di-GMP was extracted by ultrasonication, and its concentration was measured by a c-di-GMP ELISA kit (Mskbio, Beijing, China) and expressed as pmol/mg. NS represents no significant difference.
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A Fur consensus-like sequence AATAAGCATAGTTTTCATC with a weighted score of 8.1 located from −126 bp to −108 bp was detected within the upstream of the VCA0560 gene[38,52], suggesting that VCA0560 transcription might be directly regulated by Fur in V. cholerae. In a previous study, Fur has been demonstrated to repress c-di-GMP production and biofilm formation by V. cholerae independent of iron[13]. Thus, the bacterium was cultured in LB broth and then harvested to investigate the Fur-dependent transcription of VCA0560. As shown in Figure 5A, the luminescence activity under the direct action of the VCA0560 promoter was higher in Δfur than in WT across the growth periods. EMSA results indicated that His-Fur dose-dependently bound to the 581 bp upstream of the VCA0560 gene but was incapable of binding to the negative control DNA from recA (Figure 5B). DNase I footprinting assay revealed that His-Fur protected a single DNA region located from −162 bp to −19 bp upstream of VCA0560 (Figure 5C). Thus, VCA0560 transcription was directly suppressed by Fur.
Figure 5. Fur regulated the transcription of the VCA0560 gene. The first base of the start codon of VCA0650 was defined as +1. (A) Luminescence assay. The recombinant pBBRlux plasmid containing the regulatory DNA region of VCA0560 was introduced into Δfur and WT to measure the lux activity (RLU; the light units/OD600) for each strain. (B) EMSA. The [γ-32P]-ATP-labeled DNA probe of VCA0560 was incubated with different amounts of His-Fur and then analyzed by 4% (w/v) polyacrylamide gel electrophoresis. The results were detected by autoradiography. (C) DNase I footprinting. Fluorescently-labeled DNA probe of VCA0560 was incubated with different amounts of His-Fur (L-I, II, and III containing 0, 2.95, and 8.85 pmol His-Fur, respectively) and then digested with DNase I. The protected regions are marked with boxes and positions.
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An MQSR consensus-like sequence TAATTGTAGAATTATCATTA with a weighted score of 8.3 located from −46 bp to −27 bp was detected within the upstream of the VCA0560 gene[48], suggesting that VCA0560 transcription might be directly regulated by HapR. As shown in Figure 6A, VCA0560 expressed was enhanced significantly in ΔhapR compared with that in WT across the growth periods. EMSA results demonstrated that His-HapR dose-dependently bound to the regulatory DNA region of the VCA0560 gene but was incapable of binding to the negative control DNA fragment from recA (Figure 6B). DNase I footprinting assay results showed that His-HapR bound one DNA region located from −59 bp to −11 bp upstream of the coding region of VCA0560 (Figure 6C). Thus, VCA0560 transcription was directly inhibited by HapR.
Protein Containing the GGDEF Domain Affects Motility and Biofilm Formation in Vibrio cholerae and is Negatively Regulated by Fur and HapR
doi: 10.3967/bes2023.080
- Received Date: 2022-11-10
- Accepted Date: 2022-01-26
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Key words:
- Vibrio cholera /
- Cyclic di-GMP /
- VCA0560 /
- Fur /
- HapR
Abstract:
Citation: | GAO He, MA Li Zhi, QIN Qin, CUI Yao, MA Xiao Han, ZHANG Yi Quan, KAN Biao. Protein Containing the GGDEF Domain Affects Motility and Biofilm Formation in Vibrio cholerae and is Negatively Regulated by Fur and HapR[J]. Biomedical and Environmental Sciences, 2023, 36(10): 949-958. doi: 10.3967/bes2023.080 |