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苜蓿银纹夜蛾多核型多角体病毒和云杉色卷蛾多核型多角体病毒的v-cath基因以前酶原的形式表达。

Autographa californica multiple nucleopolyhedrovirus and Choristoneura fumiferana multiple nucleopolyhedrovirus v-cath genes are expressed as pre-proenzymes.

作者信息

Hodgson Jeffrey J, Arif Basil M, Krell Peter J

机构信息

Department of Molecular and Cellular Biology, University of Guelph, Guelph, ON N1G 2W1, Canada.

Laboratory for Molecular Virology, Great Lakes Forestry Centre, Sault Ste Marie, ON P6A 2E5, Canada.

出版信息

J Gen Virol. 2009 Apr;90(Pt 4):995-1000. doi: 10.1099/vir.0.007740-0. Epub 2009 Mar 4.

DOI:10.1099/vir.0.007740-0
PMID:19264635
Abstract

Intracellular processing and trafficking of the baculovirus v-cath expressed cathepsin (V-CATH), which lacks canonical targeting signals, are poorly understood. The cathepsins of Autographa californica multiple nucleopolyhedrovirus (AcMNPV), Choristoneura fumiferana multiple nucleopolyhedrovirus (CfMNPV) and most other alphabaculovirus group I nucleopolyhedroviruses have well-conserved N-termini containing overlapping chymotrypsin-cleavage (Y(11)) and myristoylation (G(12)) motifs, which are suggestive of proteolytic signal-peptide cleavage to generate proV-CATH and subsequent acylation. To determine proteolytic N-terminal processing of V-CATH, haemagglutinin epitope-coding tags were fused to the 5' and/or 3' ends of AcMNPV and CfMNPV v-cath. Immunoblot analysis suggested that a small N-terminal peptide is cleaved for both viruses, indicating that v-cath is expressed as a pre-proenzyme. The two viral homologues undergo similar proteolytic processing, but have different glycosylation or other post-translational modifications. An AcMNPV V-CATH-DsRED fusion protein co-localized to the endoplasmic reticulum with an HDEL motif-containing green fluorescent protein. Based on these findings, pre-proV-CATH processing and trafficking mechanisms are postulated.

摘要

杆状病毒v-cath表达的组织蛋白酶(V-CATH)缺乏典型的靶向信号,其细胞内加工和运输过程尚不清楚。苜蓿银纹夜蛾多粒包埋核型多角体病毒(AcMNPV)、云杉芽卷叶蛾多粒包埋核型多角体病毒(CfMNPV)以及大多数其他甲型杆状病毒属I组核型多角体病毒的组织蛋白酶具有保守性良好的N端,其中包含重叠的胰凝乳蛋白酶切割(Y(11))和肉豆蔻酰化(G(12))基序,这表明蛋白水解信号肽切割可产生前体V-CATH并随后进行酰化。为了确定V-CATH的蛋白水解N端加工过程,将血凝素表位编码标签融合到AcMNPV和CfMNPV v-cath的5'和/或3'端。免疫印迹分析表明,两种病毒的N端均切割掉了一个小肽段,这表明v-cath以前体酶原的形式表达。这两种病毒同源物经历相似的蛋白水解加工过程,但具有不同的糖基化或其他翻译后修饰。AcMNPV的V-CATH-DsRED融合蛋白与含HDEL基序的绿色荧光蛋白共定位于内质网。基于这些发现,推测了前体酶原V-CATH的加工和运输机制。

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