Abstract
Yersinia pestis, which is the causative agent of plague, has acquired exceptional pathogenicity potential during its evolution from Y. pseudotuberculosis. Two laterally acquired plasmids, namely, pMT1 and pPCP1, are specific to Y. pestis and are critical for pathogenesis and flea transmission. Small regulatory RNAs (sRNAs) commonly function as regulators of gene expression in bacteria. MicF, is a paradigmatic sRNA that acts as a post-transcriptional repressor through imperfect base pairing with the 5′-UTR of its target mRNA, ompF, in Escherichia coli. The high sequence conservation and minor variation in the RNA duplex of MicF-ompF has been reported in Yersinia. In this study, we utilized super-folder GFP reporter gene fusion to validate the post-transcriptional MicF-mediated regulation of target mRNA ompF in Y. pestis. Unexpectedly, upon MicF overexpression, the slightly upregulated expression of OmpF were found in the wild-type strain, which contradicted the previously established model. Interestingly, the translational repression of ompF target fusions was restored in the intrinsic plasmids-cured Y. pestis strain, suggesting intrinsic plasmids influence the MicF-mediated translational repression of ompF in Y. pestis. Further examination showed that plasmid pPCP1 is likely the main contributor to the abolishment of MicF-mediated translational repression of endogenous or plasmid-borne ompF. It represents that the possible roles of intrinsic plasmids should be considered upon investigating sRNA-mediated gene regulation, at least in Y. pestis, even if the exact mechanism is not fully understood.
Highlights
The human pathogenic species of Yersiniae include Yersinia pestis, Y. pseudotuberculosis, and Y. enterocolitica (Perry and Fetherston, 1997)
The Small regulatory RNAs (sRNAs) plasmid is a high-copy vector, which ensures the high level of expressed MicF and minimizes the inference of chromosome-encoded MicF
We found that the intrinsic plasmid(s) have an effect on sRNAmediated regulation, at least on the MicF-mediated ompF translation
Summary
The human pathogenic species of Yersiniae include Yersinia pestis, Y. pseudotuberculosis, and Y. enterocolitica (Perry and Fetherston, 1997). In this study we utilized super-folder GFP reporter gene fusion to validate the MicF-mediated regulation of the ompF 5′ UTR in Y. pestis. Fold changes in the MicF-mediated OmpF expression were calculated by dividing the specific fluorescence of strains with MicF overexpression by that of strains with negative control plasmid.
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