Folding of an mRNA Pseudoknot Required for Stop Codon Readthrough: Effects of Mono- and Divalent Ions on Stability

Unfolding of an mRNA pseudoknot that induces ribosome suppression of the gag gene stop codon in Moloney murine leukemia virus has been studied by UV hyperchromicity and calorimetry. The pseudoknot melts in two steps, corresponding to its two helical stems. The total enthalpy of denaturation is ∼170...

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Bibliographic Details
Published in:	Biochemistry (Easton) Vol. 36; no. 51; pp. 16173 - 16186
Main Authors:	Gluick, Thomas C, Wills, Norma M, Gesteland, Raymond F, Draper, David E
Format:	Journal Article
Language:	English
Published:	United States American Chemical Society 23-12-1997
Subjects:	Animals Calorimetry Cations, Divalent - metabolism Cations, Divalent - pharmacology Cations, Monovalent - metabolism Cations, Monovalent - pharmacology Codon, Terminator - genetics Genes, gag - genetics Metals, Alkali - pharmacology Mice Moloney murine leukemia virus - chemistry Moloney murine leukemia virus - genetics Nucleic Acid Conformation - drug effects Nucleic Acid Denaturation Quaternary Ammonium Compounds - pharmacology Ribonucleases - metabolism RNA, Messenger - chemistry RNA, Messenger - metabolism RNA, Viral - chemistry RNA, Viral - metabolism Sequence Analysis, RNA Temperature Thermodynamics Urea - pharmacology
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Summary:	Unfolding of an mRNA pseudoknot that induces ribosome suppression of the gag gene stop codon in Moloney murine leukemia virus has been studied by UV hyperchromicity and calorimetry. The pseudoknot melts in two steps, corresponding to its two helical stems. The total enthalpy of denaturation is ∼170 kcal/mol, approximately the value expected for the secondary structure. At low salt concentrations (<50 mM KCl) the unfolding transitions are not two-state, but they approach two-state behavior at higher salt concentrations. The structure is preferentially stabilized by smaller alkali metal ions (Li+ > Na+ > K+ > Rb+ > Cs+) and by NH4 +; the same preferences are exhibited by one of the stems in the context of a hairpin. Divalent metal ions are not required to fold the pseudoknot but do stabilize it further. To examine divalent ion effects over a wide concentration range, urea was used to lower the RNA unfolding temperature and was shown not to affect characteristics of the pseudoknot unfolding in other respects. The pseudoknot binds divalent ions somewhat more tightly than a hairpin but shows only weak selectivity for different size ions. It is suggested that a region of “intermediate” divalent ion binding affinity, in between highly ligated specific sites and purely delocalized ion binding in character, is created by the pseudoknot fold but that nonspecific, delocalized ion binding contributes at least half the free energy of pseudoknot stabilization by Mg2+.
Bibliography:	Abstract published in Advance ACS Abstracts, December 1, 1997. istex:82527887F4E14ADF3FD20F3D456B42CE20C3D225 ark:/67375/TPS-DPGZPD4D-G This work was supported by NIH Grant GM37005. ObjectType-Article-2 SourceType-Scholarly Journals-1 ObjectType-Feature-1 content type line 23 ObjectType-Article-1 ObjectType-Feature-2
ISSN:	0006-2960 1520-4995
DOI:	10.1021/bi971362v