Overnight cultures were diluted to an A600 nm of 30 and swabbed

Overnight cultures were diluted to an A600 nm of 3.0 and swabbed onto M9 minimal media plates. Plates included ampicillin as appropriate for the strains. Antibacterial compounds (20 μL) were spotted onto 6-mm sterile disks and placed on the plates. The plates were incubated at 37 °C for 20 h, and zones of inhibition were measured. As a control, a tetracycline disk was placed on every plate. All compounds were tested at least four separate times (biological replicates). MICs were performed as described as Wiegand et al. (2008) in 48 or 96 well plates with representative compounds used in the disk diffusion assays. Cetylpyridinium chloride (CPC) was only tested in the MIC assays as it precipitated on agar

plates. Minimal media containing glucose were used for all Gamma-secretase inhibitor experiments, and MICs were determined after 20 h of incubation at 37 °C. Strains were tested a minimum of two times. There was no variation in the MIC for a particular strain and antibacterial compound. Bacterial growth assays were initiated by inoculating M9 minimal media containing glucose with a 1 : 100 dilution of bacteria at A600 nm of 3.0. Bacteria were grown at 37 °C with shaking at 250 r.p.m. and read at A600 nm. Growth analysis was performed four times (biological replicates). Percent growth was calculated by dividing the A600 nm, in the presence of ETBR by the A600 nm in the absence

of ETBR and multiplying by 100. All statistics were performed in R (http://www.R-project.org). CAL-101 A P-value of < 0.05 was considered significant. Initially, we determined whether the presence of the dcm gene influences sugE expression. Strains expressing different levels of the dcm gene were constructed (Militello et al., 2012). These included a wild-type strain containing a plasmid with a truncated dcm gene (wild-type/pDcm-9), a wild-type strain with a functional dcm plasmid that overexpresses the dcm gene (wild-type/pDcm-21), a dcm

knockout strain with a plasmid with a truncated dcm gene (Δdcm/pDcm-9), and a dcm knockout strain with a functional dcm plasmid (Δdcm/pDcm-21). These strains were grown to early logarithmic phase and early Astemizole stationary phase, and sugE RNA levels were determined via reverse transcriptase qPCR (Table 2A). SugE RNA levels were c. 7 × higher in the dcm knockout strain with a plasmid with a truncated dcm gene at early stationary phase, and sugE RNA levels returned to normal in the dcm knockout strain with a functional dcm plasmid (complementation; P < 0.05). Thus, the presence of Dcm normally represses sugE expression at early stationary phase. At early logarithmic phase, robust up-regulation of sugE was not observed in the dcm knockout strain with a plasmid with a truncated dcm gene. Overexpression of the dcm had little effect on sugE expression at both early logarithmic and early stationary phase, and may be due to the fact that the E.

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