A PCR fragment containing the mutant cacA promoter was amplified

A PCR fragment containing the mutant cacA promoter was amplified from Salmonella chromosomal DNA using the primers 832, 833, 835, and 454 by the asymmetric PCR-based synthesis method [46] and recombined into the chromosome, replacing the tetA insertion in the strain AK1055. Strain AK1070, which harbors lacZY genes under the control of a mutant cacA promoter with two nucleotide ARN-509 solubility dmso substitutions (TCCT A CAC T to TCCT T CAC A) in the -10 region at the pgtP locus, was Foretinib constructed by a combination of the one-step gene inactivation method and the counterselection

method for Tets colonies. A PCR fragment containing the mutant cacA promoter was amplified from Salmonella chromosomal DNA using the primers 832, 833,

836, and 454 by the asymmetric PCR-based synthesis method [46] and recombined into the chromosome, replacing the tetA insertion in the strain AK1055. Strain AK1057, which harbors a deletion in the cpxA coding region, was constructed by the one-step gene inactivation method [45]. A CmR cassette was amplified from pKD3 using the primers 393 and 394 and recombined into the 14028s chromosome. Strain AK1058, LY2874455 supplier which harbors a deletion in the rssB coding region, was constructed by the one-step gene inactivation method [45]. A CmR cassette was amplified from pKD3 using the primers 367 and 368 and recombined into the 14028s chromosome. Strain AK1059, which harbors a deletion in the rpoS coding region, was constructed

by the one-step gene inactivation method [45]. A CmR cassette was amplified from pKD3 using the primers 473 and 474 and recombined into the 14028s chromosome. Strain AK1060, which harbors a deletion in the cacA coding region, was constructed by the one-step second gene inactivation method [45]. A CmR cassette was amplified from pKD3 using the primers 333 and 336 and recombined into the 14028s chromosome. Strain AK1077, which harbors a deletion in the trxA coding region, was constructed by the one-step gene inactivation method [45]. A CmR cassette was amplified from pKD3 using the primers 1160 and 1161 and recombined into the 14028s chromosome. Strain AK1078, which harbors a deletion in the trxB coding region, was constructed by the one-step gene inactivation method [45]. A CmR cassette was amplified from pKD3 using the primers 1164 and 1165 and recombined into the 14028s chromosome. Strain AK1079, which harbors a deletion in the trxC coding region, was constructed by the one-step gene inactivation method [45]. A CmR cassette was amplified from pKD3 using the primers 1166 and 1167 and recombined into the 14028s chromosome. Plasmid construction The pBAD18-cacA plasmid, encoding the CacA protein, was constructed by cloning a PCR fragment, generated using the primers 337 and 338 from a pWN1 template, between the EcoRI and BamHI sites in the pBAD18plasmid.

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