Literature DB >> 19642681

Matching active site and substrate structures for an RNA editing reaction.

Subhash Pokharel1, Prasanna Jayalath, Olena Maydanovych, Rena A Goodman, Selina C Wang, Dean J Tantillo, Peter A Beal.   

Abstract

The RNA-editing adenosine deaminases (ADARs) catalyze deamination of adenosine to inosine in a double-stranded structure found in various RNA substrates, including mRNAs. Here we present recent efforts to define structure/activity relationships for the ADAR reaction. We describe the synthesis of new phosphoramidites for the incorporation of 7-substituted-8-aza-7-deazaadenosine derivatives into RNA. These reagents were used to introduce the analogues into mimics of the R/G-editing site found in the pre-mRNA for the human glutamate receptor B subunit (GluR B). Analysis of the kinetics of the ADAR2 reaction with analogue-containing RNAs indicated 8-aza-7-deazaadenosine is an excellent substrate for this enzyme with a deamination rate eight times greater than that for adenosine. However, replacing the C7 hydrogen in this analogue with bromine, iodine, or propargyl alcohol failed to increase the deamination rate further but rather decreased the rate. Modeling of nucleotide binding in the enzyme active site suggested amino acid residues that may be involved in nucleotide recognition. We carried out a functional screen of a library of ADAR2 mutants expressed in S. cerevisiae that varied the identity of these residues to identify active deaminases with altered active sites. One of these mutants (ADAR2 R455A) was able to substantially overcome the inhibitory effect of the bulky C7 substituents (-Br, -I, propargyl alcohol). These results advance our understanding of the importance of functional groups found in the edited nucleotide and the role of specific active site residues of ADAR2.

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Year:  2009        PMID: 19642681     DOI: 10.1021/ja9034076

Source DB:  PubMed          Journal:  J Am Chem Soc        ISSN: 0002-7863            Impact factor:   15.419


  17 in total

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3.  RNA-Seq analysis identifies a novel set of editing substrates for human ADAR2 present in Saccharomyces cerevisiae.

Authors:  Tristan Eifler; Subhash Pokharel; Peter A Beal
Journal:  Biochemistry       Date:  2013-10-31       Impact factor: 3.162

4.  A Phenotypic Screen for Functional Mutants of Human Adenosine Deaminase Acting on RNA 1.

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Journal:  ACS Chem Biol       Date:  2015-09-22       Impact factor: 5.100

5.  The components of xRNA: synthesis and fluorescence of a full genetic set of size-expanded ribonucleosides.

Authors:  Armando R Hernández; Eric T Kool
Journal:  Org Lett       Date:  2011-01-07       Impact factor: 6.005

6.  A Fluorescent Adenosine Analogue as a Substrate for an A-to-I RNA Editing Enzyme.

Authors:  Rena A Mizrahi; Dongwon Shin; Renatus W Sinkeldam; Kelly J Phelps; Andrea Fin; Dean J Tantillo; Yitzhak Tor; Peter A Beal
Journal:  Angew Chem Int Ed Engl       Date:  2015-06-10       Impact factor: 15.336

7.  7-Substituted 8-aza-7-deazaadenosines for modification of the siRNA major groove.

Authors:  José M Ibarra-Soza; Alexi A Morris; Prasanna Jayalath; Hayden Peacock; Wayne E Conrad; Michael B Donald; Mark J Kurth; Peter A Beal
Journal:  Org Biomol Chem       Date:  2012-07-05       Impact factor: 3.876

8.  Probing RNA recognition by human ADAR2 using a high-throughput mutagenesis method.

Authors:  Yuru Wang; Peter A Beal
Journal:  Nucleic Acids Res       Date:  2016-09-09       Impact factor: 16.971

9.  Potent and selective inhibition of A-to-I RNA editing with 2'-O-methyl/locked nucleic acid-containing antisense oligoribonucleotides.

Authors:  Rena A Mizrahi; Nicole T Schirle; Peter A Beal
Journal:  ACS Chem Biol       Date:  2013-02-21       Impact factor: 5.100

10.  A screening protocol for identification of functional mutants of RNA editing adenosine deaminases.

Authors:  Tristan Eifler; Dalen Chan; Peter A Beal
Journal:  Curr Protoc Chem Biol       Date:  2012-12-01
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