In addition to its role as a repressor of anfA, MopA has an exclusive role in activating the mop gene, which codes for a Mo-binding molbindin (Wiethaus et al., 2006, 2009). MopB does not substitute for MopA in mop activation. MopA and MopB binding to Mo-boxes is enhanced by Mo (Wiethaus et al., 2006). As the anfA-Mo-box overlaps the transcription start site, binding of MopA or MopB is thought to prevent binding of RNA polymerase. In contrast, the mop-Mo-box precedes the putative RNA polymerase-binding site, and thus,
MopA and RNA polymerase probably bind side by side to activate mop transcription. It is unclear why MopB MAPK Inhibitor Library clinical trial is unable to bind the Mo-box upstream of mop. Like R. capsulatus, Azotobacter vinelandii, Haemophilus influenzae, and Rhodopseudomonas
palustris have two ModE homologues (Larimer et al., 2004; Pau, 2004; Hernandez et al., 2009). The A. vinelandii modE Selleckchem Buparlisib copy located between the modG molbindin and the modABC transport genes mediates Mo repression of modABC, vnfA (coding for the activator of vanadium nitrogenase genes), and anfA (Mouncey et al., 1995, 1996; Premakumar et al., 1998). To date, however, detailed analyses of Mo-boxes serving as ModE-binding sites have not been carried out in any of these species. In the present study, we investigated the contributions of individual nucleotides of the anfA-Mo-box and the mop-Mo-box on Mo-dependent gene regulation in R. capsulatus. Specific single-base substitutions were shown to be sufficient to considerably diminish repression of anfA, enhance mop activation, or even completely abolish mop activation. The bacterial strains and plasmids used in this study are listed in Table 1. Conjugational plasmid transfer from E. coli S17-1 to R. capsulatus, molybdenum-free minimal medium (AK-NL), growth conditions, and antibiotic concentrations were described previously Pembrolizumab cost (Sicking et al., 2005). A 388-bp
DNA fragment carrying the wild-type anfA promoter was PCR amplified with the primer pair 5′-CCAGGATTCGAGCTTGTGCCGCCG-3′/5′-CCGGCATTCGCCGGTGAAGCACTG-3′ using R. capsulatus total DNA as a template. In parallel, a 353-bp DNA fragment carrying the wild-type mop promoter was PCR amplified with the primer pair 5′-CCGCCGTCTGGATCTGCCGCTCTC-3′/5′-TCGGCGGCGGCTTCGTTGGTGAT-3′. PCR products were cloned into pBluescript KS, resulting in plasmids pLP1 and pLP14 (Table 1), which subsequently served as templates for site-directed mutagenesis of the anfA-Mo-box (Fig. 1b) and the mop-Mo-box (Fig. 1c), respectively. Single-base substitutions within the Mo-boxes were generated following the QuikChange protocol (Stratagene, Amsterdam, the Netherlands). The resulting pBluescript derivatives carrying mutant anfA and mop promoters are listed in Table 1. BamHI–HindIII fragments obtained from pBluescript derivatives carrying anfA and mop promoter variants with single-base substitutions (Fig.