To separate cells in pellicle and underneath, cultures were withd

To separate cells in pellicle and underneath, cultures were withdrawn carefully for collecting planktonic cells and the left pellicles. For growth measurement, 27 parallel starting cultures were used and 3 were collected at each

time point and the rest remained undisturbed. The cell density (OD600) of cultures containing planktonic cells was measured first as the planktonic cell density and measured again as the overall cell density after cells from pellicles were added and extensively vortexed. To quantify the pellicles formed by the S. oneidensis wild-type and mutant strains, cells from pellicles AZD5153 cell line were collected, suspended in 30 ml fresh LB, violently vortexed, and applied to the spectrometer at 600 nm. Proteinase K and DNase I treatment of S. oneidensis pellicles S. oneidensis was statically cultured in LB broth with the addition of proteinase K (0 μg/mL, 100 μg/mL, and 500 μg/mL) or DNase I (Qiagen, 0U/mL, 100U/mL, 500U/mL and 1000U/mL) for 3 days [55]. We also investigated whether these 3 enzymes could dissolve established pellicles. 2-day old pellicles were rinsed this website with 20 mM Tris-HCl (pH = 8.0) and incubated in the same buffer supplemented with proteinase K at 37°C for 2 days. Similarly, 2-day old pellicles were incubated with DNase I to examine

the DNA content at room temperature for 2 days. Mutagenesis, physiological characterization and complementation of the

resulting mutants Deletion mutation strains were constructed using the fusion PCR method illustrated previously [56]. Primers used for mutagenesis were listed in Additional file 1. In brief, two DNA fragments flanking Florfenicol the target gene were generated from S. oneidensis genomic DNA by PCR with primers 5F/5R and 3F/3R, respectively. Fusion PCR was then performed to join these two DNA fragments with primers 5F/3R. The resulting single buy Dasatinib fragment was digested with SacI and ligated into the SacI-digested and phosphatase-treated suicide vector pDS3.0. The resultant vectors were electroporated into the donor strain, E. coli WM3064 and then moved to S. oneidensis by conjugation. Integration of the mutagenesis construct into the chromosome and resolution were performed to generate the final deletion strains. The deletion was verified by PCR and DNA sequencing. For complementation, DNA fragments containing aggA or flgA were generated by PCR amplification with MR-1 genomic DNA as the template using primers SO4320-COM-F/SO3988-COM-R and SO3253-COM-F/SO3253-COM-R, respectively as listed in Additional file 1. These fragments were digested with SacI and ligated to SacI-digested pBBR1MCS-5 to form pBBR-AGGA and pBBR-FLGA, which was electroporated into WM3064.

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