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通过生物信息学分析和诱变鉴定神经坏死病毒B2中与双链RNA结合及抑制RNA干扰活性相关的关键残基。

Identification of critical residues in nervous necrosis virus B2 for dsRNA-binding and RNAi-inhibiting activity through by bioinformatic analysis and mutagenesis.

作者信息

Ou Ming-Chang, Chen Young-Mao, Jeng Mei-Fen, Chu Chiau-Jun, Yang Huey-Lang, Chen Tzong-Yueh

机构信息

Laboratory of Molecular Genetics, Institute of Biotechnology, College of Bioscience and Biotechnology, National Cheng Kung University, Tainan 701, Taiwan.

出版信息

Biochem Biophys Res Commun. 2007 Sep 28;361(3):634-40. doi: 10.1016/j.bbrc.2007.07.075. Epub 2007 Jul 24.

DOI:10.1016/j.bbrc.2007.07.075
PMID:17669362
Abstract

It is known that the non-structural B2 protein of nervous necrosis virus (NNV) plays an important role in viral replication and can inhibit the RNA interference system of the host cell. Moreover, the mechanism of NNV B2 protein to inhibit RNAi is by sequestration and protection of double strand (ds) RNA. In the flock house virus (FHV), a model alphanodavirus, the structural and mutational analysis of B2 identified that the positively charged Arg54 of the alpha2 helix mediated the dsRNA-binding activity. According to the betanodavirus B2 protein alignment and modeling results, the amino acid sequences and the predicted structure of betanodavirus B2 are different from alphanodaviruses. It was suggested that the four Arg residues of alpha3 helix between amino residues 52-60 of B2 may be involved in dsRNA-binding activity. Thus, this study replaced these four Arg residues with Gln at position 52 (R52Q), 53 (R53Q), 59 (R59Q), and 60 (R60Q) by site-directed mutagenesis method. The dsRNA-binding assays of these B2 mutants demonstrated that mB2(R53Q) and mB2(R60Q) mutants are dsRNA-binding defective. Moreover, we have found mB2(R53Q) and mB2(R60Q) could not antagonize RNAi by using HeLa cell as an RNAi inhibition model. These results suggested that Arg53 and Arg60 of betanodavirus B2 protein may be similar to Arg54 of alphanodavirus FHV B2 protein and are critical for dsRNA binding and RNAi-inhibiting. This study may serve as an example where bioinformatic analysis of related viral genomes may lead to meaningful structural and functional clues for certain viral proteins.

摘要

已知神经坏死病毒(NNV)的非结构B2蛋白在病毒复制中起重要作用,并可抑制宿主细胞的RNA干扰系统。此外,NNV B2蛋白抑制RNAi的机制是通过螯合和保护双链(ds)RNA。在家禽舍病毒(FHV,一种甲型诺达病毒模型)中,对B2的结构和突变分析表明,α2螺旋带正电荷的Arg54介导了dsRNA结合活性。根据乙型诺达病毒B2蛋白的比对和建模结果,乙型诺达病毒B2的氨基酸序列和预测结构与甲型诺达病毒不同。有人提出,B2氨基酸残基52-60之间α3螺旋的四个Arg残基可能参与dsRNA结合活性。因此,本研究通过定点诱变方法将这四个Arg残基在位置52(R52Q)、53(R53Q)、59(R59Q)和60(R60Q)处替换为Gln。这些B2突变体的dsRNA结合试验表明,mB2(R53Q)和mB2(R60Q)突变体存在dsRNA结合缺陷。此外,我们发现以HeLa细胞作为RNAi抑制模型时,mB2(R53Q)和mB2(R60Q)不能拮抗RNAi。这些结果表明,乙型诺达病毒B2蛋白的Arg53和Arg60可能与甲型诺达病毒FHV B2蛋白的Arg54相似,对dsRNA结合和RNAi抑制至关重要。本研究可作为一个例子,说明对相关病毒基因组的生物信息学分析可能为某些病毒蛋白带来有意义的结构和功能线索。

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