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伯尔尼病毒纤突蛋白的一级结构和翻译后加工

Primary structure and post-translational processing of the Berne virus peplomer protein.

作者信息

Snijder E J, Den Boon J A, Spaan W J, Weiss M, Horzinek M C

机构信息

Institute of Virology, Veterinary Faculty, State University of Utrecht, The Netherlands.

出版信息

Virology. 1990 Oct;178(2):355-63. doi: 10.1016/0042-6822(90)90332-l.

Abstract

The nucleotide sequence of the peplomer (P) protein gene of Berne virus (BEV), the torovirus prototype, was determined. The gene encodes an apoprotein of 1581 amino acids with an Mr of about 178K. The open reading frame was cloned behind the T7 RNA polymerase promoter and its translation product was identified as the BEV P protein precursor by in vivo expression and immunoprecipitation. The deduced amino acid sequence contains a number of domains which are typical for type I membrane glycoproteins: an N-terminal signal sequence, a putative C-terminal transmembrane anchor, and a cytoplasmic tail. Eighteen potential N-glycosylation sites, two heptad repeat domains, and a possible "trypsin-like" cleavage site were identified. The mature P protein consists of two subunits and their electrophoretic mobility upon endoglycosidase F treatment strongly suggests that the predicted cleavage site is functional in vivo. The heptad repeat domains are probably involved in the generation of an intra-chain coiled-coil secondary structure; similar inter-chain interactions can play a role in P protein oligomerization. Using a sucrose gradient assay the P protein was indeed shown to form dimers. The intra- and inter-chain coiled-coil interactions may stabilize the elongated BEV peplomers.

摘要

测定了环曲病毒原型——伯尔尼病毒(BEV)纤突(P)蛋白基因的核苷酸序列。该基因编码一个含1581个氨基酸的脱辅基蛋白,分子量约为178K。将开放阅读框克隆到T7 RNA聚合酶启动子之后,通过体内表达和免疫沉淀鉴定其翻译产物为BEV P蛋白前体。推导的氨基酸序列包含一些典型的I型膜糖蛋白结构域:一个N端信号序列、一个推定的C端跨膜锚定区和一个胞质尾。鉴定出18个潜在的N糖基化位点、两个七肽重复结构域和一个可能的“类胰蛋白酶”切割位点。成熟的P蛋白由两个亚基组成,经内切糖苷酶F处理后其电泳迁移率强烈表明预测的切割位点在体内具有功能。七肽重复结构域可能参与链内卷曲螺旋二级结构的形成;类似的链间相互作用可能在P蛋白寡聚化中起作用。使用蔗糖梯度分析确实表明P蛋白形成二聚体。链内和链间的卷曲螺旋相互作用可能稳定延长的BEV纤突。

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