单纯疱疹病毒 1 型外壳蛋白 VP22 的病毒粒子整合是由反式高尔基体网络定位促进的,并且不依赖于与糖蛋白 E 的相互作用。
Virion incorporation of the herpes simplex virus type 1 tegument protein VP22 is facilitated by trans-Golgi network localization and is independent of interaction with glycoprotein E.
机构信息
Fox Chase Cancer Center, Program in Immune Cell Development and Host Defense, Philadelphia, PA 19111, USA.
出版信息
Virology. 2010 Sep 15;405(1):176-92. doi: 10.1016/j.virol.2010.06.007. Epub 2010 Jun 26.
Abstract
HSV-1 virions contain a proteinaceous layer termed the tegument that lies between the nucleocapsid and viral envelope. The molecular mechanisms that facilitate incorporation of tegument proteins are poorly characterized. The tegument protein VP22 interacts with VP16 and the cytoplasmic tail of glycoprotein E (gE). Virion incorporation of VP22 occurs independently of interaction with VP16; however, the contribution of gE binding remains undefined. Site-directed mutagenesis was used to identify VP22 mutants which abrogate interaction with gE but retain VP16 binding. Virion incorporation assays demonstrated that failure to bind gE did not abrogate VP22 packaging. A region of VP22 which binds to both VP16 and gE failed to be packaged efficiently, with wild-type levels of incorporation only attained when residues 43-86 of VP22 were present. Mutational analysis of an acidic cluster of amino acids within this region indicates that this motif facilitates trans-Golgi network (TGN) localization and optimal virion incorporation of VP22.
摘要
单纯疱疹病毒 1 病毒粒子包含一个蛋白层,称为被膜,位于核衣壳和病毒包膜之间。促进被膜蛋白掺入的分子机制尚未得到很好的描述。被膜蛋白 VP22 与 VP16 和糖蛋白 E(gE)的细胞质尾巴相互作用。VP22 的病毒粒子掺入不依赖于与 VP16 的相互作用;然而,gE 结合的贡献仍未定义。定点突变用于鉴定 VP22 突变体,这些突变体消除了与 gE 的相互作用,但保留了与 VP16 的结合。病毒粒子掺入测定表明,不与 gE 结合不会阻止 VP22 的包装。与 VP16 和 gE 结合的 VP22 区域未能有效地被包装,只有当 VP22 的残基 43-86 存在时,才能达到野生型的掺入水平。对该区域内一个酸性氨基酸簇的突变分析表明,该基序有助于跨高尔基网络(TGN)定位和 VP22 的最佳病毒粒子掺入。
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Herpesvirus assembly: an update.疱疹病毒组装:最新进展。
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