Literature DB >> 14581474

Evaluation of the RNA determinants for bacterial and yeast RNase III binding and cleavage.

Bruno Lamontagne1, Sherif Abou Elela.   

Abstract

Bacterial double-stranded RNA-specific RNase III recognizes the A-form of an RNA helix with little sequence specificity. In contrast, baker yeast RNase III (Rnt1p) selectively recognizes NGNN tetraloops even when they are attached to a B-form DNA helix. To comprehend the general mechanism of RNase III substrate recognition, we mapped the Rnt1p binding signal and directly compared its substrate specificity to that of both Escherichia coli RNase III and fission yeast RNase III (PacI). Rnt1p bound but did not cleave long RNA duplexes without NGNN tetraloops, whereas RNase III indiscriminately cleaved all RNA duplexes. PacI cleaved RNA duplexes with some preferences for NGNN-capped RNA stems under physiological conditions. Hydroxyl radical footprints indicate that Rnt1p specifically interacts with the NGNN tetraloop and its surrounding nucleotides. In contrast, Rnt1p interaction with GAAA-capped hairpins was weak and largely unspecific. Certain duality of substrate recognition was exhibited by PacI but not by bacterial RNase III. E. coli RNase III recognized RNA duplexes longer than 11 bp with little specificity, and no specific features were required for cleavage. On the other hand, PacI cleaved long, but not short, RNA duplexes with little sequence specificity. PacI cleavage of RNA stems shorter than 27 bp was dependent on the presence of an UU-UC internal loop two nucleotides upstream of the cleavage site. These observations suggest that yeast RNase IIIs have two recognition mechanisms, one that uses specific structural features and another that recognizes general features of the A-form RNA helix.

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Year:  2003        PMID: 14581474     DOI: 10.1074/jbc.M309324200

Source DB:  PubMed          Journal:  J Biol Chem        ISSN: 0021-9258            Impact factor:   5.157


  28 in total

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4.  Structure of a yeast RNase III dsRBD complex with a noncanonical RNA substrate provides new insights into binding specificity of dsRBDs.

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5.  The pseudouridine synthase RluD is required for normal ribosome assembly and function in Escherichia coli.

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6.  Beyond secondary structure: primary-sequence determinants license pri-miRNA hairpins for processing.

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9.  A new alpha-helical extension promotes RNA binding by the dsRBD of Rnt1p RNAse III.

Authors:  Nicolas Leulliot; Sophie Quevillon-Cheruel; Marc Graille; Herman van Tilbeurgh; Thomas C Leeper; Katherine S Godin; Thomas E Edwards; Snorri T L Sigurdsson; Natasha Rozenkrants; Roland J Nagel; Manuel Ares; Gabriele Varani
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10.  The catalytic efficiency of yeast ribonuclease III depends on substrate specific product release rate.

Authors:  Marc-Andre Comeau; Daniel A Lafontaine; Sherif Abou Elela
Journal:  Nucleic Acids Res       Date:  2016-06-01       Impact factor: 16.971

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