g., nitrofurantoin), generating highly reactive electrophilic intermediates [23]. While the physiological role of nitroreductases
in bacteria is unknown, mutants lacking nitroreductases are more resistant to nitroaromatic compounds [24]. Since the loss of gene function is associated with an increase in resistance to the antimicrobial agent, we thought that these genes might provide an ideal starting point for studying spontaneous mutation, as mutations in these genes would not be biased by the constraints of having to retain enzymatic function. We used database learn more searches to identify a potential nitroreductase in GC, cloned and expressed the gene, verified its biochemical properties, and analyzed the DNA sequence of the gene in spontaneous nitrofurnatoin-resistant mutants. Methods Bacterial strains and growth media E. coli strain DH5α-mcr was used for genetic manipulations and was obtained from Bethesda Research Laboratories [now Life Technologies] (Rockville, MD). N. gonorrhoeae strains used in this study are described in Table 1. N. gonorrhoeae were grown
on GCK agar (GCMB, Difco supplemented with 0.5% GSK126 mw agar and Kellogg’s supplements) [25]. GCP broth was prepared by adding proteose peptone #3 (15 g), soluble starch (1 g), KH2PO4 (4 g), K2HPO4 (1 g), NaCl (5 g)/L of ultra-pure water (pH 7.5). LB agar and broth were prepared from powder obtained from US Biologicals. Plasmids used in this study are described in Table 2. Table 1 Bacterial
strains used in these studies Strain Relevant Phenotype Source N. gonorrhoeae FA1090 P. Frederick Sparling N. gonorrhoeae FA19 William Shafer N. gonorrhoeae F62 P. Frederick Sparling N. gonorrhoeae MS11 Herman Schneider N. gonorrhoeae PID2 Herman Schneider N. gonorrhoeae FA1090(M1) Spontaneous nitrofurantoin resistant mutant This Study N. gonorrhoeae FA1090 -Nfsb(mod) Strain with a modified poly adenine tract in the beginning of the gene This Study N. gonorrhoeae FA1090 NfsB-BsmI-Σ Strain lacking NfsB This Study Table 2 Plasmids used in these studies Plasmids Properties Cobimetinib manufacturer Source pK18 General cloning vector [38] pHP45Σ Plasmid containing the Σ interposon [39] pNFSB The nfsB selleck region from FA1090 was amplified by PCR using primers NP1 and NP2. The amplicon was purified, digested with BamHI and cloned into the BamHI site in pK18. This study pEC1 The DNA between the adjacent BsmI sites were removed by digesting pEC2 with BsmI, ligating the DNA and transforming it into E. coli. This study pEC2 Two BsmI sites were inserted into pNFSB by PCR amplification using primers NfsBBsmI-3F and -2R, treating the amplicon with S1 nuclease and polynucleotide kinase, ligating the DNA and transforming it into E. coli. This study pEC3 A BsrGI site was introduced downstream of the NfsB coding sequence by PCR amplification of pEC1 using primers dwnstrm-F and dwnstrm-R.