, 2009). pLM100 with the mutY gene and pLM102 with the mutM gene were electroporated into PAOMY-Mgm separately as previously described (Mandsberg et al., 2009). The method was modified after Oliver (Oliver et al., 2000). To determine
the mutant frequency (MF) to rifampicin and streptomycin, an overnight culture of 20 mL LB media was centrifuged for 10 min at 6000 g, and resuspended in 1 mL of 0.9% NaCl. Serial dilutions of the bacterial culture were made, and 100 μL of appropriate dilution was spread on LB, 300 mg L−1 rifampicin and 500 mg L−1 streptomycin. The plates were incubated at 37 °C for 36 h before the CFU was determined. The CFU on GSK126 rifampicin and streptomycin plates were compared with the CFU from LB plates. At least five replicates were run for each experiment. The MRs are estimated using a fluctuation experiment, where a culture of each strain was diluted to 2 × 104 cells in 280 μL of LB and grown in 27 microtitre wells to stationary phase, then plated on 100 mg L−1 rifampicin LB agar plates to count the number of mutants. Three wells for each strain were used to estimate the CFU per
well. The expected number of mutations per well was then estimated using the Ma—Sandri—Sarkar (MSS) maximum likelihood method described by Sarkar et al. (1992). The MR was found by dividing the number of mutations by APO866 mw the final CFU per well. The MIC was determined on 105 CFU mL−1 using the E-test system (AB Biodisk, Solna, Sweden), according to instructions of the manufacturer. Experiments were run at least in triplicates. To isolate ciprofloxacin resistant mutants, overnight cultures of PAO1 and PAOMY-Mgm were diluted and plated on 5% blood agar plates containing twofold dilutions of ciprofloxacin (Bagge et al., 2000; Mandsberg et al., 2009). Isolated resistant colonies were grown in LB without antibiotic, twice before E-test was performed with 100 μL of 10−4 dilution of an overnight culture. The strains were cultured in LB to an OD600nm = 1.0. Four millilitres of each culture was harvested, and RNA isolation and purification were performed using RNA Protect Sodium butyrate Bacteria
Reagent and RNeasy Mini Kit (Qiagen, Hilden, Germany). RQ1 RNAse free DNAse (Promega, Madison, WI) was added to remove contaminating DNA. The experiment was run in triplicates. Processing of the P. aeruginosa GeneChip (Affymetrix) was performed at the Department of Clinical Biochemistry, Microarray Core Unit, Rigshospitalet, University of Copenhagen, Denmark. The gene expression analysis was done using arraystar v.3 Software (DNASTAR), http://isim.ku.dk/units/ub/research/paoym_vs_pao1microarray.pdf/. The level of expression of mexB, mexD, mexF and mexX was determined using real-time PCR in adapted isolates from the growth competition assays, and the level of expression of pfpI and PA5148 was determined to verify the microarray data. RNA from the logarithmic phase growth OD600 nm = 0.
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