The mixtures were incubated at 37°C for 1 hour and were then transferred to ice to halt any additional growth. The samples were mixed by repeated pipetting just before plating 20 μl to LB agar plates. The plates were then incubated overnight at 37°C and the number of viable microbial cells for each H2O2 concentration was determined by colony forming
unit (CFU) counting. For SB202190 supplier HOCl-mediated killing, 5 × 108 bacterial cells were aliquotted, in duplicate, to 15 ml conical tubes at a final volume of 1 ml of DPBS containing various MEK inhibitor concentrations of HOCl as indicated. The tubes were incubated at 37°C for 1 hour with agitation and were then placed on ice. The samples were then passed through 25 gauge needles. Bacterial samples were then diluted 1:105 in DPBS. Fifty microliters of each diluted sample was plated to LB agar and cultured at 37°C. Microbial viability was assessed by CFU counting. Assessing HOCl- and H2O2-induced bacterial membrane permeability Permeability of bacterial membranes after exposure of the organisms to reagent HOCl or H2O2 was measured using the LIVE/DEAD BacLight Bacterial Viability and Counting Kit (Molecular Probes, Carlsbad, CA). For HOCl-mediated membrane permeability studies,
PsA, SA, KP, BC, and EC were grown in LB broth medium at 37°C overnight and subsequently subcultured (1:100) in fresh LB media until the culture reached late-log phase. The cells selleck compound were then pelleted and washed with DPBS, quantified, and resuspended to 6.67 × 109 cells per milliliter. Cells (5 × 108) were aliquotted to 15 ml conical
tubes, and reagent NaOCl was added to the final concentrations indicated. The bacterial suspensions were incubated with the oxidant for 1 hour at 37°C and 220 rpm. The samples were placed on ice. Finally, the bacteria were pelleted in a table-top centrifuge at full speed for 2 minutes, and pellets were washed with ice-cold DPBS. The samples were stained according to manufacturer protocol with the vital dye Syto 9 as well as with propidium Non-specific serine/threonine protein kinase iodide (PI) which stains permeabilized cells. The percentages of fluorescently stained intact and permeable cells were assessed by flow cytometry, and the data were normalized to the oxidant-free controls. Controls for intact and permeable bacteria were produced by 1 hour incubation with either 0.85% NaCl or 70% ethanol, respectively, followed by washing and resuspension in 0.85% NaCl. For H2O2-mediated membrane permeability studies, 1.25 × 106 cells were used per sample, each in a volume of 50 ml of DPBS to preserve the same cell density as was used in the above described CFU viability assay. Incubation times were the same as for the HOCl membrane permeability experiments. After incubation, the 50 ml samples were concentrated to 1 ml by centrifugation at 3000 × g for 15 minutes followed by washing, staining, and analysis as described above for HOCl assays.