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蝙蝠源流感 A 病毒神经氨酸酶样分子 N10 的结构与功能表征

Structural and functional characterization of neuraminidase-like molecule N10 derived from bat influenza A virus.

机构信息

School of Life Sciences, University of Science and Technology of China, Hefei 230027, China.

出版信息

Proc Natl Acad Sci U S A. 2012 Nov 13;109(46):18897-902. doi: 10.1073/pnas.1211037109. Epub 2012 Sep 24.

Abstract

The recent discovery of the unique genome of influenza virus H17N10 in bats raises considerable doubt about the origin and evolution of influenza A viruses. It also identifies a neuraminidase (NA)-like protein, N10, that is highly divergent from the nine other well-established serotypes of influenza A NA (N1-N9). The structural elucidation and functional characterization of influenza NAs have illustrated the complexity of NA structures, thus raising a key question as to whether N10 has a special structure and function. Here the crystal structure of N10, derived from influenza virus A/little yellow-shouldered bat/Guatemala/153/2009 (H17N10), was solved at a resolution of 2.20 Å. Overall, the structure of N10 was found to be similar to that of the other known influenza NA structures. In vitro enzymatic assays demonstrated that N10 lacks canonical NA activity. A detailed structural analysis revealed dramatic alterations of the conserved active site residues that are unfavorable for the binding and cleavage of terminally linked sialic acid receptors. Furthermore, an unusual 150-loop (residues 147-152) was observed to participate in the intermolecular polar interactions between adjacent N10 molecules of the N10 tetramer. Our study of influenza N10 provides insight into the structure and function of the sialidase superfamily and sheds light on the molecular mechanism of bat influenza virus infection.

摘要

最近在蝙蝠中发现了流感病毒 H17N10 的独特基因组,这让人对甲型流感病毒的起源和进化产生了相当大的怀疑。它还鉴定了一种神经氨酸酶(NA)样蛋白 N10,该蛋白与其他 9 种已确立的甲型流感 NA(N1-N9)高度不同。流感 NAs 的结构阐明和功能表征说明了 NA 结构的复杂性,因此提出了一个关键问题,即 N10 是否具有特殊的结构和功能。在这里,我们从流感病毒 A/小黄肩蝙蝠/危地马拉/153/2009(H17N10)中获得了 N10 的晶体结构,分辨率为 2.20Å。总体而言,N10 的结构被发现与其他已知的流感 NA 结构相似。体外酶促测定表明,N10 缺乏典型的 NA 活性。详细的结构分析揭示了保守活性位点残基的剧烈改变,不利于末端连接的唾液酸受体的结合和切割。此外,观察到一个不寻常的 150 环(残基 147-152)参与相邻 N10 分子之间的分子间极性相互作用,形成 N10 四聚体。我们对流感 N10 的研究提供了对唾液酸酶超家族结构和功能的深入了解,并阐明了蝙蝠流感病毒感染的分子机制。

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