Regulation of 6S RNA biogenesis by switching utilization of both sigma factors and endoribonucleases
In Escherichia coli, 6S RNA functions as a modulator of RNA polymerase sigma(70)-holoenzyme activity, but its biosynthetic pathway remains uncharacterized. In this study, to further understand the regulatory circuit of 6S RNA biosynthesis for the modulation of Esigma(70) activity, we have characterized the biogenesis of 6S RNA. We reveal that there are two different precursors, a long and a short molecule, which are transcribed from the distal P2 and proximal P1 promoter, respectively. Transcription from the P2 promoter is both sigma(70)- and sigma(S)-dependent, whereas, in contrast, P1 transcription is sigma(70)- but not sigma(S)-dependent. Both precursors are processed to generate the 5' end of 6S RNA, and while the long precursor is processed exclusively by RNase E, the short precursor is processed by both RNase G and RNase E. Our data indicate that the switching of the utilization of both sigma factors and endoribonucleases in the biogenesis of 6S RNA would play an essential role in modulating its levels in E.coli.
- Publisher
- OXFORD UNIV PRESS
- Issue Date
- 2004
- Language
- English
- Article Type
- Article
- Keywords
COLI-RNPB PROMOTER; ESCHERICHIA-COLI; RIBOSOMAL-RNA; M1 RNA; RIBONUCLEASE-P; STRINGENT RESPONSE; ENCODING GENES; CAFA PROTEIN; STABLE RNAS; 10SA RNA
- Citation
NUCLEIC ACIDS RESEARCH, v.32, no.20, pp.6057 - 6068
- ISSN
- 0305-1048
- Appears in Collection
- CH-Journal Papers(저널논문)
- Files in This Item
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