[32]. Briefly, PI3K inhibitor the upstream and downstream DNA sequence that flanks (about 500 bp each) the operon targeted for deletion were cloned into pGPISce-I. This suicide plasmid contains a unique restriction site for the endonuclease I-SceI. Mutagenesis plasmids were mobilized by conjugation into B. cenocepacia J2315 where they integrate into the chromosome by homologous OSI-906 solubility dmso recombination. Exconjugants were selected in the presence of trimethoprim (800 μg/ml) and the single crossover insertion of the
mutagenic plasmid in the B. cenocepacia genome was confirmed by PCR analysis. Subsequently, a second plasmid, pDAISce-I (encoding the I-SceI endonuclease) was introduced by conjugation. Site-specific double-strand breaks take place in the chromosome at the I-SceI recognition site, resulting in tetracycline-resistant (due to the presence of pDAI-SceI) and learn more trimethoprim-susceptible (indicating
the loss of the integrated mutagenic plasmid) exconjugants. PCR amplifications of flanking regions for the construction of the mutagenesis plasmids were performed with the HotStar HiFidelity Polymerase kit (Qiagen), and the specific amplifications conditions were optimized for each primer pair, as indicated in Table 3. For the deletion of the rnd-1 operon, we used KO1XL- KO1BL and KO1BR-KO1KR primer pairs [Table 3]. The PCR see more fragments were first cloned into the pGEM-T Easy vector (Promega) and the resulting plasmids were digested with XbaI-BamHI and BamHI-KpnI, respectively. The
recovered fragments were cloned together into pGPISce-I digested with XbaI and KpnI, resulting in pOP1/pGPI-SceI plasmid. For the deletion of the rnd-3 operon, PCR amplifications of flanking regions were performed using the primer pair OP13LX-OP13LB and OP13RB-OP13RE [Table 3] and the fragments were again cloned into pGEM-T Easy. After digestion with XbaI-BamHI and BamHI-EcoRI, respectively, the fragments were cloned into pGPISce-I digested with XbaI and EcoRI, resulting in pOP3/pGPI-SceI plasmid. For the deletion of the rnd-4 operon, PCR amplifications of flanking regions were performed using KO4XL-KO4NL and KO4NR-KO4KR primers [Table 3]. After cloning into pGEM-T Easy and digestion with XbaI-NdeI and NdeI-KpnI, respectively, the fragments were cloned into pGPISce-I digested with XbaI and KpnI, resulting in pOP4/pGPI-SceI plasmid.