3, upper circle graph). This was a surprising finding since it is well documented that transcription of nitrogen fixation genes (fix/nif) is oxygen-regulated in legume nodules and only induced under microoxic conditions in free-living bacteria [38]. Nonetheless, it has been also reported that a moderate decrease of the ambient oxygen concentration (to 5%) in the gas phase over a culture is sufficient to trigger ATP-dependent

autophosphorylation of the deoxygenated FixL hemoprotein in the FixLJ-FixK phosphorelay cascade [39]. In S. meliloti phosphorylated FixJ not only activates transcription of the fixK1/K2 regulatory genes but also of nifA, the transcriptional activator of the nif genes specifying the nitrogenase complex. Expression of nifA has been shown to demand more stringent microaerobic conditions [38]. Therefore, selleck screening library down-regulation of the fix genes in the hfq mutant can be only explained if our culture conditions (15-ml test tubes) enabled some level of expression of fixK1/fixK2 in

the learn more wild-type 1021 strain and the accumulation of the corresponding transcripts is influenced by the lack of Hfq. Indeed, β-galactosidase assays in the wild-type 1021 strain carrying a fixK::lacZ transcriptional fusion demonstrated a 4-fold induction of fixK transcription in our culture conditions PLX3397 in vivo compared to better aerated cultures (i.e. 20-ml cultures in 100-ml Loperamide Erlenmeyer flasks). Similar experiments with a nifA::lacZ transcriptional fusion revealed no signs of transcription of nifA whatever the aeration of the culture (not shown). These findings and the fact that nifA expression had been also shown to be influenced by Hfq in other α-proteobacterial diazotrophs [23–26] prompted us to further investigate the effects of Hfq on both nifA and fixK expression

in more stringent microaerobic conditions by RT-PCR (Fig. 6). Confirming the results of microarray experiments FixK transcripts were readily detected in RNA from wild-type bacteria grown under assumed aerobiosis (Fig. 6; line 1), whereas the 1021Δhfq failed to accumulate these transcripts in these culture conditions (Fig. 6; line 2). As expected, after 4 hours incubation in a microoxic atmosphere (2% O2) wild-type fixK expression was clearly induced as compared to aerobiosis (Fig. 6; compare lines 1 and 3). Strikingly, similar amounts of the FixK transcript were detected in the RNA from the hfq mutant extracted after the same treatment (Fig. 6; line 4). In contrast, nifA expression was only detected after bacterial incubation in microaerobiosis (Fig 6; line 3), further confirming that transcription of this gene demands lower O2 concentrations than fixK.