Recognition of duplex RNA by the deaminase domain of the RNA editing enzyme ADAR2

被引:38
|
作者
Phelps, Kelly J. [1 ]
Tran, Kiet [1 ]
Eifler, Tristan [1 ]
Erickson, Anna I. [2 ]
Fisher, Andrew J. [1 ,2 ]
Beal, Peter A. [1 ]
机构
[1] Univ Calif Davis, Dept Chem, Davis, CA 95616 USA
[2] Univ Calif Davis, Dept Mol & Cellular Biol, Davis, CA 95616 USA
基金
美国国家卫生研究院;
关键词
DOUBLE-STRANDED-RNA; GLUR-B; ADENOSINE DEAMINASES; IN-VITRO; BINDING; SITE; MUTATIONS; ANALOGS; PROTEIN; ACT;
D O I
10.1093/nar/gku1345
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Adenosine deaminases acting on RNA (ADARs) hydrolytically deaminate adenosines (A) in a wide variety of duplex RNAs and misregulation of editing is correlated with human disease. However, our understanding of reaction selectivity is limited. ADARs are modular enzymes with multiple double-stranded RNA binding domains (dsRBDs) and a catalytic domain. While dsRBD binding is understood, little is known about ADAR catalytic domain/RNA interactions. Here we use a recently discovered RNA substrate that is rapidly deaminated by the isolated human ADAR2 deaminase domain (hADAR2-D) to probe these interactions. We introduced the nucleoside analog 8-azanebularine (8-azaN) into this RNA (and derived constructs) to mechanistically trap the protein-RNA complex without catalytic turnover for EMSA and ribonuclease footprinting analyses. EMSA showed that hADAR2-D requires duplex RNA and is sensitive to 2 '-deoxy substitution at nucleotides opposite the editing site, the local sequence and 8-azaN nucleotide positioning on the duplex. Ribonuclease V1 footprinting shows that hADAR2-D protects similar to 23 nt on the edited strand around the editing site in an asymmetric fashion (similar to 18 nt on the 5 ' side and similar to 5 nt on the 3 ' side). These studies provide a deeper understanding of the ADAR catalytic domain-RNA interaction and new tools for biophysical analysis of ADAR-RNA complexes.
引用
收藏
页码:1123 / 1132
页数:10
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