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鉴定融合(F)蛋白三聚体上影响介导细胞间融合的 F 蛋白血凝素-神经氨酸酶特异性的结构域。

Identification of domains on the fusion (F) protein trimer that influence the hemagglutinin-neuraminidase specificity of the f protein in mediating cell-cell fusion.

机构信息

Department of Microbiology and Molecular Genetics, Mie University Graduate School of Medicine, 2-174 Edobashi, Tsu, Mie 514-8507, Japan.

出版信息

J Virol. 2011 Apr;85(7):3153-61. doi: 10.1128/JVI.01666-10. Epub 2011 Jan 26.

Abstract

For most paramyxoviruses, virus type-specific interaction between fusion (F) protein and attachment protein (hemagglutinin-neuraminidase [HN], hemagglutinin [H], or glycoprotein [G]) is a prerequisite for mediating virus-cell fusion and cell-cell fusion. Our previous cell-cell fusion assay using the chimeric F proteins of human parainfluenza virus 2 (HPIV2) and simian virus 41 (SV41) suggested that the middle region of the HPIV2 F protein contains the site(s) that determines its specificity for the HPIV2 HN protein. In the present study, we further investigated the sites of the F protein that could be critical for determining the HN protein specificity. By analyzing the reported structure of the F protein of parainfluenza virus 5 (PIV5), we found that four major domains (M1, M2, M3, and M4) and five minor domains (A to E) in the middle region of the PIV5 F protein were exposed on the trimer surface. We then replaced these domains with the SV41 F counterparts individually or in combination and examined whether the resulting chimeras could mediate cell-cell fusion when coexpressed with the SV41 HN protein. The results showed that a chimera designated M(1+2), which harbored SV41 F-derived domains M1 and M2, mediated cell-cell fusion with the coexpressed SV41 HN protein, suggesting that these domains are involved in determining the HN protein specificity. Intriguingly, another chimera which harbored the SV41 F-derived domain B in addition to domains M1 and M2 showed increased specificity for the SV41 HN protein compared to that of M(1+2), although it was capable of mediating cell-cell fusion by itself.

摘要

对于大多数副黏病毒而言,病毒融合(F)蛋白与黏附蛋白(血凝素神经氨酸酶[HN]、血凝素[H]或糖蛋白[G])之间的特定型别相互作用是介导病毒-细胞融合和细胞-细胞融合的前提。我们之前使用人副流感病毒 2(HPIV2)和猿猴病毒 41(SV41)嵌合 F 蛋白进行的细胞-细胞融合试验表明,HPIV2 F 蛋白的中部区域包含决定其对 HPIV2 HN 蛋白特异性的位点。在本研究中,我们进一步研究了对决定 HN 蛋白特异性至关重要的 F 蛋白位点。通过分析副流感病毒 5(PIV5)F 蛋白的报告结构,我们发现 PIV5 F 蛋白中部的四个主要结构域(M1、M2、M3 和 M4)和五个次要结构域(A 至 E)暴露在三聚体表面。然后,我们分别或以组合的方式用 SV41 F 蛋白的对应结构域替换这些结构域,并检查当与 SV41 HN 蛋白共表达时,产生的嵌合体能否介导细胞-细胞融合。结果表明,指定为 M(1+2)的嵌合体与共表达的 SV41 HN 蛋白介导细胞-细胞融合,表明这些结构域参与决定 HN 蛋白的特异性。有趣的是,另一个嵌合体除了包含 M1 和 M2 外还包含 SV41 F 衍生的结构域 B,与 M(1+2)相比,它对 SV41 HN 蛋白的特异性增加,尽管它本身能够介导细胞-细胞融合。

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