The CafA Protein Required for the 5′-Maturation of 16 S rRNA Is a 5′-End-dependent Ribonuclease That Has Context-dependent Broad Sequence Specificity
| Autor: | Mark R. Tock, Gregory Carroll, Kenneth J. McDowall, Andrew P. Walsh |
|---|---|
| Rok vydání: | 2000 |
| Předmět: |
Untranslated region
RNase P E-site Biochemistry Chromatography Affinity Substrate Specificity RNA interference RNA Ribosomal 16S Endoribonucleases RNA Precursors RNA Antisense RNA Messenger Ribonuclease RNA Processing Post-Transcriptional RNA Small Interfering Molecular Biology Messenger RNA biology Escherichia coli Proteins RNA Cell Biology Ribosomal RNA Molecular biology Cell biology RNA Bacterial RNA Ribosomal 23S Exoribonucleases biology.protein Bacterial Outer Membrane Proteins |
| Zdroj: | Journal of Biological Chemistry. 275:8726-8732 |
| ISSN: | 0021-9258 |
| Popis: | The CafA protein, which was initially described as having a role in either Escherichia coli cell division or chromosomal segregation, has recently been shown to be required for the maturation of the 5'-end of 16 S rRNA. The sequence of CafA is similar to that of the N-terminal ribonucleolytic half of RNase E, an essential E. coli enzyme that has a central role in the processing of rRNA and the decay of mRNA and RNAI, the antisense regulator of ColE1-type plasmids. We show here that a highly purified preparation of CafA is sufficient in vitro for RNA cutting. We detected CafA cleavage of RNAI and a structured region from the 5'-untranslated region of ompA mRNA within segments cleavable by RNaseE, but not CafA cleavage of 9 S RNA at its "a" RNase E site. The latter is consistent with the finding that the generation of 5 S rRNA from its 9 S precursor can be blocked by inactivation of RNase E in cells that are wild type for CafA. Interestingly, however, a decanucleotide corresponding in sequence to the a site of 9 S RNA was cut efficiently indicating that cleavage by CafA is regulated by the context of sites within structured RNAs. Consistent with this notion is our finding that although 23 S rRNA is stable in vivo, a segment from this RNA is cut efficient by CafA at multiple sites in vitro. We also show that, like RNase E cleavage, the efficiency of cleavage by CafA is dependent on the presence of a monophosphate group on the 5'-end of the RNA. This finding raises the possibility that the context dependence of cleavage by CafA may be due at least in part to the separation of a cleavable sequence from the 5'-end of an RNA. Comparison of the sites surrounding points of CafA cleavage suggests that this enzyme has broad sequence specificity. Together with the knowledge that CafA can cut RNAI and ompA mRNA in vitro within segments whose cleavage in vivo initiates the decay of these RNAs, this finding suggests that CafA may contribute at some point during the decay of many RNAs in E. coli. |
| Databáze: | OpenAIRE |
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