Ble for sporadic food-borne cholera in the summer [21]. Environmental V. cholerae isolates (RGVCs) collected at two locations along the Rio Grande were examined to test whether constitutive T6SS expression is prevalent in V. cholerae exposed to microbial competitors and predators.Materials and Methods Strains and Culture ConditionsA streptomycin-resistant V. cholerae strain V52 (O37 serogroup) MedChemExpress Hexokinase II Inhibitor II, 3-BP lacking hapA, rtxA, and hlyA genes [4] was used as a T6SS-positive strain in all experiments presented in this study. DH5alpir and SM10lpir were used for cloning, and mating of pWM91-based plasmids, respectively. The strains and plasmids used in this study are listed in Table 1. Unless stated otherwise, bacteria were grown in a Luria-Bertani (LB) broth at 37uC with shaking (200 rpm). Rifampicin-resistant (50 mg?mL21) Vibrio 1485-00-3 communis, Vibrio harveyi,Strain or plasmid Strains Vibrio cholerae 23727046 V52 Vibrio cholerae V52DvasK DL2111, DL2112, DL4211, DL4215 DL4211 DvasK DL4215 DvasK Escherichia coli DH5a lpirDescriptionReference or sourceO37 serogroup strain, DhapA, DrtxA, DhlyA, smR V52 mutant lacking vasK (VCA0120) Environmental isolates collected in this study (see Table 3). DL4211 mutant lacking vasK (VCA0120) DL4215 mutant lacking vasK (VCA0120) fhuA2 D(argF-lacZ)U169 phoA glnV44 W80 D(lacZ)M15 gyrA96 recA1 relA1 endA1 thi-1 hsdR17 KmR, thi-1, thr, leu, tonA, lacY, supE, recA::RP4-2-Tc::Mu, pir F- lambda- ilvG- rfb-50 rph-1, RifR Wild-type. T6SS-negative control[25] [25] This study This study This study Provenzano Laboratory (University of Texas at Brownsville) Mekalanos Laboratory (Harvard Medical School) Raivio Laboratory (University of Alberta) Kessin Laboratory (Columbia University)Escherichia coli SM10lpir Escherichia coli MG1655 Klebsiella pneumoniae Plasmids pBAD18 pBAD18-vasH::myc pBAD24 pBAD24-vasK pWM91 pGEM-T-easy doi:10.1371/journal.pone.0048320.tpBAD vector, pBR322 ori, araC, KanR pBAD18 carrying vasH (VCA0117) of the Vibrio cholerae strain V52 pBAD vector, pBR322 ori, araC, AmpR pBAD24 carrying vasK (VCA0120) of the Vibrio cholerae strain V52 oriR6K mobRP4 lacI ptac tnp mini-Tn10Km; Kmr Ampr Vector for cloning PCR products, AmpR[39] [16] [39] [6] [23] PromegaCompetition Mechanisms of V. choleraeTable 2. Primers.PRIMER 59vasH 39-vasH-myc 59-vasK-pBAD24 39-vasK-pBAD24 59-16S Universal (E8F) 39-16S Universal (U1115R)OLIGONUCLEOTIDE SEQUENCE (restriction sites underlined) GAATTCACCATGAGTCAATGGCTGGCG CCTCTAGATCATAAATCTTCTTCAGAAATTAATTTTTGTTCTGGGGTTTTGATCTCCAA TTTGAATTCACCATGTGGAAATTCATT TTTTCTAGATTAATAGAGTGTTTTAGAC AGAGTTTGATCCTGGCTCAG AGGGTTGCGCTCGTTGdoi:10.1371/journal.pone.0048320.tand Pseudoalteromonas phenolica were grown in K YTSS broth (2.5 g?L21 tryptone, 4 g?L21 yeast extract, 20 g?L21 sea salts (Sigma)) at 30uC. Antibiotic concentrations used to maintain the plasmids were 100 mg?mL21 ampicillin or 50 mg?mL21 kanamycin. D. discoideum AX3 cells were obtained from the Dicty Stock Center and maintained in liquid culture (HL5) with shaking (150 rpm) at 22uC [22]. Environmental bacteria were collected by submerging a Turtox tow net (Envco, New Zealand) with a 20 mm pore-size Nitex mesh spanning a 30.48 cm diameter mouth in estuary water for one minute. Water samples (200 mL) collected from estuaries of the Rio Grande delta were blended with a handheld homogenizer (PRO Scientific; Oxford, CT), and vacuum filtered through Whatman filter paper number 3 (GE Healthcare, Little Chalfont, UK). A second vacuum filtration was performed on the filt.Ble for sporadic food-borne cholera in the summer [21]. Environmental V. cholerae isolates (RGVCs) collected at two locations along the Rio Grande were examined to test whether constitutive T6SS expression is prevalent in V. cholerae exposed to microbial competitors and predators.Materials and Methods Strains and Culture ConditionsA streptomycin-resistant V. cholerae strain V52 (O37 serogroup) lacking hapA, rtxA, and hlyA genes [4] was used as a T6SS-positive strain in all experiments presented in this study. DH5alpir and SM10lpir were used for cloning, and mating of pWM91-based plasmids, respectively. The strains and plasmids used in this study are listed in Table 1. Unless stated otherwise, bacteria were grown in a Luria-Bertani (LB) broth at 37uC with shaking (200 rpm). Rifampicin-resistant (50 mg?mL21) Vibrio communis, Vibrio harveyi,Strain or plasmid Strains Vibrio cholerae 23727046 V52 Vibrio cholerae V52DvasK DL2111, DL2112, DL4211, DL4215 DL4211 DvasK DL4215 DvasK Escherichia coli DH5a lpirDescriptionReference or sourceO37 serogroup strain, DhapA, DrtxA, DhlyA, smR V52 mutant lacking vasK (VCA0120) Environmental isolates collected in this study (see Table 3). DL4211 mutant lacking vasK (VCA0120) DL4215 mutant lacking vasK (VCA0120) fhuA2 D(argF-lacZ)U169 phoA glnV44 W80 D(lacZ)M15 gyrA96 recA1 relA1 endA1 thi-1 hsdR17 KmR, thi-1, thr, leu, tonA, lacY, supE, recA::RP4-2-Tc::Mu, pir F- lambda- ilvG- rfb-50 rph-1, RifR Wild-type. T6SS-negative control[25] [25] This study This study This study Provenzano Laboratory (University of Texas at Brownsville) Mekalanos Laboratory (Harvard Medical School) Raivio Laboratory (University of Alberta) Kessin Laboratory (Columbia University)Escherichia coli SM10lpir Escherichia coli MG1655 Klebsiella pneumoniae Plasmids pBAD18 pBAD18-vasH::myc pBAD24 pBAD24-vasK pWM91 pGEM-T-easy doi:10.1371/journal.pone.0048320.tpBAD vector, pBR322 ori, araC, KanR pBAD18 carrying vasH (VCA0117) of the Vibrio cholerae strain V52 pBAD vector, pBR322 ori, araC, AmpR pBAD24 carrying vasK (VCA0120) of the Vibrio cholerae strain V52 oriR6K mobRP4 lacI ptac tnp mini-Tn10Km; Kmr Ampr Vector for cloning PCR products, AmpR[39] [16] [39] [6] [23] PromegaCompetition Mechanisms of V. choleraeTable 2. Primers.PRIMER 59vasH 39-vasH-myc 59-vasK-pBAD24 39-vasK-pBAD24 59-16S Universal (E8F) 39-16S Universal (U1115R)OLIGONUCLEOTIDE SEQUENCE (restriction sites underlined) GAATTCACCATGAGTCAATGGCTGGCG CCTCTAGATCATAAATCTTCTTCAGAAATTAATTTTTGTTCTGGGGTTTTGATCTCCAA TTTGAATTCACCATGTGGAAATTCATT TTTTCTAGATTAATAGAGTGTTTTAGAC AGAGTTTGATCCTGGCTCAG AGGGTTGCGCTCGTTGdoi:10.1371/journal.pone.0048320.tand Pseudoalteromonas phenolica were grown in K YTSS broth (2.5 g?L21 tryptone, 4 g?L21 yeast extract, 20 g?L21 sea salts (Sigma)) at 30uC. Antibiotic concentrations used to maintain the plasmids were 100 mg?mL21 ampicillin or 50 mg?mL21 kanamycin. D. discoideum AX3 cells were obtained from the Dicty Stock Center and maintained in liquid culture (HL5) with shaking (150 rpm) at 22uC [22]. Environmental bacteria were collected by submerging a Turtox tow net (Envco, New Zealand) with a 20 mm pore-size Nitex mesh spanning a 30.48 cm diameter mouth in estuary water for one minute. Water samples (200 mL) collected from estuaries of the Rio Grande delta were blended with a handheld homogenizer (PRO Scientific; Oxford, CT), and vacuum filtered through Whatman filter paper number 3 (GE Healthcare, Little Chalfont, UK). A second vacuum filtration was performed on the filt.