Amino acid residue doublet propensity in the protein-RNA interface and its application to RNA interface prediction

被引:100
作者
Kim, Oanh T. P.
Yura, Kei [1 ]
Go, Nobuhiro
机构
[1] Japan Atom Energy Agcy, Quantum Bioinformat Team, Ctr Computat Sci & Engn, Kizu, Kyoto 6190215, Japan
[2] Japan Atom Energy Agcy, Computat Biol Grp, Quantum Beam Sci Directorate, Kizu, Kyoto 6190215, Japan
[3] Japan Atom Energy Agcy, JST, CREST, Kizu, Kyoto 6190215, Japan
[4] Japan Atom Energy Agcy, Res Unit Quantum Beam Life Sci Initiat, Quantum Beam Sci Directorate, Kizu, Kyoto 6190215, Japan
[5] Nara Inst Sci & Technol, Bioinformat Unit, Nara 6300196, Japan
关键词
D O I
10.1093/nar/gkl819
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
Protein-RNA interactions play essential roles in a number of regulatory mechanisms for gene expression such as RNA splicing, transport, translation and post-transcriptional control. As the number of available protein-RNA complex 3D structures has increased, it is now possible to statistically examine protein-RNA interactions based on 3D structures. We performed computational analyses of 86 representative protein-RNA complexes retrieved from the Protein Data Bank. Interface residue propensity, a measure of the relative importance of different amino acid residues in the RNA interface, was calculated for each amino acid residue type (residue singlet interface propensity). In addition to the residue singlet propensity, we introduce a new residue-based propensity, which gives a measure of residue pairing preferences in the RNA interface of a protein (residue doublet interface propensity). The residue doublet interface propensity contains much more information than the sum of two singlet propensities alone. The prediction of the RNA interface using the two types of propensities plus a position-specific multiple sequence profile can achieve a specificity of about 80%. The prediction method was then applied to the 3D structure of two mRNA export factors, TAP (Mex67) and UAP56 (Sub2). The prediction enables us to point out candidate RNA interfaces, part of which are consistent with previous experimental studies and may contribute to elucidation of atomic mechanisms of mRNA export.
引用
收藏
页码:6450 / 6460
页数:11
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