Further work is necessary to investigate this attractive possibility. Analysis of the S. pneumoniae RNase R genomic region revealed the presence of several ORFs that may be part of a large transcript shown to be mainly expressed under cold-shock. Some of them are essential for growth, as it is the case of the GTP-binding protein Era and of the Compound C Dephospho-CoA ARN-509 concentration kinase. Others are important in the resistance to some drugs or mutagens, as for instance formamidopyrimidine-DNA glycosylase, the multi-drug
resistance efflux pump PmrA and the tellurite resistance protein TehB. The first gene of this large operon – YbeY, a putative metalloprotease – appears to be essential for translation under high temperature growth conditions. However, besides RNase R and SmpB none of these genes have known links to cold-stress. smpB is located downstream of rnr and we show that both genes are co-transcribed. Although we were not able to identify an active promoter immediately upstream of rnr or smpB that could drive the transcription of these genes independently, a promoter upstream of secG was identified. secG is a small ORF located immediately upstream of rnr and transcription from its promoter is likely to drive expression of the downstream genes. Indeed, we have demonstrated that this promoter
is active and most probably drives the coupled transcription of secG, rnr and smpB. Identification of processing sites in
CRT0066101 manufacturer the overlapping region between rnr and smpB indicates that this message is processed, yielding either rnr or smpB. The fact that the coding regions of these genes overlap makes it impossible to have simultaneously both mature mRNAs. Thus, processing of the original transcript always results in disruption of one of the mRNAs. This is in agreement with our results and substantiates the hypothesis of Resveratrol the mutual dependency observed between SmpB and RNase R. In terms of cell physiology it is very interesting to note that when the cell is in need of RNase R and raises its production, the higher amount of enzyme lowers the levels of smpB mRNA. Since SmpB destabilizes RNase R, by lowering the amount of SmpB, the cell guarantees that RNase R will not be degraded. The fact that smpB mRNA is disrupted when rnr mRNA is matured adds another level of regulation to this complex system. On the other hand when SmpB is required, not only RNase R is destabilized, but its mRNA is also disrupted. Comparison of the rnr genomic region of different Gram-negative and Gram-positive bacteria revealed that this genomic organization (secG, rnr, smpB) seems to be a common feature among Gram-positive bacteria (Table 1). The rnr gene is clustered with secG and smpB in numerous bacteria. Does this close localization have a biological meaning? It is known that bacterial genes involved in the same pathway are frequently co-localized [40].