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水疱性口炎病毒的蛋白激酶和磷酸化蛋白

Protein kinase and phosphoproteins of vesicular stomatitis virus.

作者信息

Imblum R L, Wagner R R

出版信息

J Virol. 1974 Jan;13(1):113-24. doi: 10.1128/JVI.13.1.113-124.1974.

Abstract

Protein kinases of similar but not identical activity were found associated with vesicular stomatitis (VS) virions grown in mouse L cells, primary chicken embryo (CE) cells, and BHK-21 cells, as well as being present in VS virions grown in HeLa and Aedes albopictus cells. The virion kinase preferentially phosphorylated the nucleocapsid NS protein in vitro and to a lesser extent the envelope M protein. Other virion proteins were phosphorylated in vitro only after drastic detergent treatment. Partial evidence that the virion kinase is of cellular origin was obtained by finding reduced enzyme activity in virions released from cells pretreated with actinomycin D and cycloheximide. Selective detergent and detergent-salt fractionation of VS virions revealed that the kinase activity was present in the envelope but not the spikes. The virion kinase activity in a Triton-salt-solubilized envelope fraction could be separated from M and G proteins and partially purified by phosphocellulose column chromatography. Virions released from L, CE, and BHK-21 cells infected in the presence of [(32)P]orthophosphate were labeled almost exclusively in the NS protein. Both soluble and nucleocapsid-associated NS phosphoprotein were present in cytoplasmic extracts of VS viral-infected L cells. The origin and function of the NS phosphoprotein remain to be elucidated.

摘要

在小鼠L细胞、原代鸡胚(CE)细胞和BHK - 21细胞中生长的水泡性口炎(VS)病毒粒子以及在HeLa细胞和白纹伊蚊细胞中生长的VS病毒粒子中,发现了活性相似但不完全相同的蛋白激酶。病毒粒子激酶在体外优先磷酸化核衣壳NS蛋白,对包膜M蛋白的磷酸化程度较低。其他病毒粒子蛋白只有在经过剧烈的去污剂处理后才在体外被磷酸化。通过发现从用放线菌素D和放线菌酮预处理的细胞释放的病毒粒子中酶活性降低,获得了病毒粒子激酶起源于细胞的部分证据。对VS病毒粒子进行选择性去污剂和去污剂 - 盐分级分离表明,激酶活性存在于包膜中而不存在于刺突中。Triton - 盐溶解的包膜部分中的病毒粒子激酶活性可以与M和G蛋白分离,并通过磷酸纤维素柱色谱法进行部分纯化。在[(32)P]正磷酸盐存在下感染的L、CE和BHK - 21细胞释放的病毒粒子几乎只在NS蛋白中被标记。VS病毒感染的L细胞的细胞质提取物中同时存在可溶性和与核衣壳相关的NS磷蛋白。NS磷蛋白的起源和功能仍有待阐明。

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