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单纯疱疹病毒 UL16 和 UL21 衣壳蛋白的相互作用结构域。

Interaction domains of the UL16 and UL21 tegument proteins of herpes simplex virus.

机构信息

Department of Microbiology and Immunology, The Pennsylvania State University College of Medicine, Hershey, PA 17033, USA.

出版信息

J Virol. 2010 Mar;84(6):2963-71. doi: 10.1128/JVI.02015-09. Epub 2009 Dec 30.

Abstract

The UL16 protein of herpes simplex virus is capsid associated and was previously identified as a binding partner of the membrane-associated UL11 tegument protein (J. S. Loomis, R. J. Courtney, and J. W. Wills, J. Virol. 77:11417-11424, 2003). In those studies, a less-prominent, approximately 65-kDa binding partner of unknown identity was also observed. Mass spectrometry studies have now revealed this species to be UL21, a tegument protein that has been implicated in the transport of capsids in the cytoplasm. The validity of the mass spectrometry results was tested in a variety of coimmunoprecipitation and glutathione S-transferase pull-down experiments. The data revealed that UL21 and UL16 can form a complex in the absence of other viral proteins, even when the assays used proteins purified from Escherichia coli. Moreover, UL11 was able to pull down UL21 only when UL16 was present, suggesting that all three proteins can form a complex. Deletion analyses revealed that the second half of UL21 (residues 268 to 535) is sufficient for the UL16 interaction and packaging into virions; however, attempts to map a subdomain of UL16 were largely unsuccessful, with only the first 40 (of 373) residues being found to be dispensable. Nevertheless, it is clear that UL16 must have two distinct binding sites, because covalent modification of its free cysteines with N-ethylmaleimide blocked binding to UL11 but not UL21. These findings should prove useful for elucidating the molecular machinery used to transmit a signal into a virion when it attaches to cells, a recently discovered mechanism in which UL16 is a central player.

摘要

单纯疱疹病毒的 UL16 蛋白与衣壳相关,先前被鉴定为膜相关 UL11 衣壳蛋白的结合伴侣(J. S. Loomis、R. J. Courtney 和 J. W. Wills,J. Virol. 77:11417-11424, 2003)。在这些研究中,还观察到一种不太突出的、大约 65 kDa 的未知身份的结合伴侣。质谱研究现已表明,这种物质是 UL21,它是一种衣壳蛋白,与细胞质中衣壳的运输有关。在各种共免疫沉淀和谷胱甘肽 S-转移酶下拉实验中测试了质谱结果的有效性。数据表明,即使在使用从大肠杆菌中纯化的蛋白质进行的测定中,UL21 和 UL16 也可以在没有其他病毒蛋白的情况下形成复合物。此外,只有当 UL16 存在时,UL11 才能下拉 UL21,这表明这三种蛋白质可以形成复合物。缺失分析表明,UL21 的后半部分(残基 268 至 535)足以与 UL16 相互作用并包装到病毒粒子中;然而,试图对 UL16 的亚结构域进行作图在很大程度上不成功,只有前 40 个(373 个中的)残基是可有可无的。尽管如此,很明显 UL16 必须有两个不同的结合位点,因为其游离半胱氨酸与 N-乙基马来酰亚胺的共价修饰阻断了与 UL11 的结合,但不阻断与 UL21 的结合。这些发现应该有助于阐明当病毒颗粒附着到细胞时传递信号进入病毒颗粒所使用的分子机制,这是最近发现的一种机制,其中 UL16 是一个核心参与者。

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