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从紧邻N端的p6*蛋白上切割出1型人类免疫缺陷病毒蛋白酶,对于高效的Gag多聚蛋白加工和病毒感染性至关重要。

Cleavage of human immunodeficiency virus type 1 proteinase from the N-terminally adjacent p6* protein is essential for efficient Gag polyprotein processing and viral infectivity.

作者信息

Tessmer U, Kräusslich H G

机构信息

Heinrich-Pette-Institut, Hamburg, Germany.

出版信息

J Virol. 1998 Apr;72(4):3459-63. doi: 10.1128/JVI.72.4.3459-3463.1998.

Abstract

Maturation of infectious human immunodeficiency virus (HIV) particles requires proteolytic cleavage of the structural polyproteins by the viral proteinase (PR), which is itself encoded as part of the Gag-Pol polyprotein. Expression of truncated PR-containing sequences in heterologous systems has mostly led to the autocatalytic release of an 11-kDa species of PR which is capable of processing all known cleavage sites on the viral precursor proteins. Relatively little is known about cleavages within the nascent virus particle, on the other hand, and controversial results concerning the active PR species inside the virion and the relative activities of extended PR species have been reported. Here, we report that HIV type 1 (HIV-1) particles of four different strains obtained from different cell lines contain an 11-kDa PR, with no extended PR proteins detectable. Furthermore, mutation of the N-terminal PR cleavage site leading to production of an N-terminally extended 17-kDa PR species caused a severe defect in Gag polyprotein processing and a complete loss of viral infectivity. We conclude that N-terminal release of PR from the HIV-1 polyprotein is essential for viral replication and suggest that extended versions of PR may have a transient function in the proteolytic cascade.

摘要

传染性人类免疫缺陷病毒(HIV)颗粒的成熟需要病毒蛋白酶(PR)对结构多聚蛋白进行蛋白水解切割,而PR本身是作为Gag-Pol多聚蛋白的一部分编码的。在异源系统中表达含截短PR的序列大多会导致一种11 kDa的PR自动催化释放,该PR能够处理病毒前体蛋白上所有已知的切割位点。另一方面,对于新生病毒颗粒内的切割了解相对较少,并且关于病毒粒子内活性PR种类以及延伸PR种类的相对活性的报道存在争议。在此,我们报告从不同细胞系获得的四种不同毒株的1型HIV(HIV-1)颗粒含有一种11 kDa的PR,未检测到延伸的PR蛋白。此外,N端PR切割位点的突变导致产生N端延伸的17 kDa PR种类,这在Gag多聚蛋白加工中造成严重缺陷并导致病毒感染性完全丧失。我们得出结论,HIV-1多聚蛋白中PR的N端释放对于病毒复制至关重要,并表明PR的延伸版本可能在蛋白水解级联反应中具有短暂功能。

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