Characterization of RNA sequence determinants and antideterminants of processing reactivity for a minimal substrate of Escherichia coli ribonuclease III
Open Access
- 28 July 2006
- journal article
- Published by Oxford University Press (OUP) in Nucleic Acids Research
- Vol. 34 (13) , 3708-3721
- https://doi.org/10.1093/nar/gkl459
Abstract
Members of the ribonuclease III family are the primary agents of double-stranded (ds) RNA processing in prokaryotic and eukaryotic cells. Bacterial RNase III orthologs cleave their substrates in a highly site-specific manner, which is necessary for optimal RNA function or proper decay rates. The processing reactivities of Escherichia coli RNase III substrates are determined in part by the sequence content of two discrete double-helical elements, termed the distal box (db) and proximal box (pb). A minimal substrate of E.coli RNase III, muR1.1 RNA, was characterized and used to define the db and pb sequence requirements for reactivity and their involvement in cleavage site selection. The reactivities of muR1.1 RNA sequence variants were examined in assays of cleavage and binding in vitro. The ability of all examined substitutions in the db to inhibit cleavage by weakening RNase III binding indicates that the db is a positive determinant of RNase III recognition, with the canonical UA/UG sequence conferring optimal recognition. A similar analysis showed that the pb also functions as a positive recognition determinant. It also was shown that the ability of the GC or CG bp substitution at a specific position in the pb to inhibit RNase III binding is due to the purine 2-amino group, which acts as a minor groove recognition antideterminant. In contrast, a GC or CG bp at the pb position adjacent to the scissile bond can suppress cleavage without inhibiting binding, and thus act as a catalytic antideterminant. It is shown that a single pb+db 'set' is sufficient to specify a cleavage site, supporting the primary function of the two boxes as positive recognition determinants. The base pair sequence control of reactivity is discussed within the context of new structural information on a post-catalytic complex of a bacterial RNase III bound to the cleaved minimal substrate.Keywords
This publication has 49 references indexed in Scilit:
- Structural Insight into the Mechanism of Double-Stranded RNA Processing by Ribonuclease IIICell, 2006
- The double‐stranded RNA‐binding motif, a versatile macromolecular docking platformThe FEBS Journal, 2005
- The double-stranded-RNA-binding motif: interference and much moreNature Reviews Molecular Cell Biology, 2004
- Evaluation of the RNA Determinants for Bacterial and Yeast RNase III Binding and CleavagePublished by Elsevier ,2004
- New and old roles of the double-stranded RNA-binding domainJournal of Structural Biology, 2002
- A Network of Heterogeneous Hydrogen Bonds in GNRA TetraloopsJournal of Molecular Biology, 1996
- Characterization of the rnc-97 mutation of RNAaseIII: a glycine to glutamate substitution increases the requirement for magnesium ionsJournal of General Microbiology, 1993
- Complete nucleotide sequence of bacteriophage T7 DNA and the locations of T7 genetic elementsJournal of Molecular Biology, 1983
- Sequence-specific interaction of R17 coat protein with its ribonucleic acid binding siteBiochemistry, 1983
- Escherichia coli ribonuclease III cleavage sitesCell, 1982