OVERLAPPING PROMOTERS FOR 2 DIFFERENT RNA-POLYMERASE HOLOENZYMES CONTROL BRADYRHIZOBIUM-JAPONICUM NIFA EXPRESSION

The Bradyrhizobium japonicum NifA protein, the central regulator for nitrogen fixation gene expression, is encoded in the fixRnifA operon. This operon is activated during free-living anaerobic growth and in the symbiotic root nodule bacteroid state. In addition, it is expressed in aerobic conditions, albeit at a low level. Here, we report that this pattern of expression is due to the presence of two overlapping promoters: fixRp(1), which is of the -24/-12 class recognized by the RNA polymerase o(54), and fixRp(2),, which shares homology with the -35 and -10 regions found in other putative B. japonicum housekeeping promoters. Primer extension analyses showed that fixRp(1) directed the synthesis of a transcript, P1, that starts 12 nucleotides downstream of the -12 region. In addition to o(54), P1 was dependent on NifA and low oxygen tension. Transcripts originating from fixRp(2) started at two sites: one coincided with P1, while the most abundant, P2, initiated just two nucleotides further downstream of P1. Expression from fixRp(2) was dependent on the upstream -68 promoter region, a region known to bind a putative activator protein, but it was independent of o(54) and NifA. This promoter was expressed in aerobic and anaerobic conditions but was not expressed in 30-day-old bacteroids. Mutations in the conserved -12 region for the o(54) promoter did not show any transcript, because these mutations also disrupted the overlapping -10 region of the firRp(2) promoter. Conversely, mutations at the -24 region only affected the o(54)-dependent P1 transcript, having no effect on the expression of P2. In the absence of o(54), anaerobic expression from the fixRp(2), promoter was enhanced threefold, suggesting that in the wild-type strain, the two RNA polymerase holoenzymes must compete for binding to the same promoter region.