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活性人类免疫缺陷病毒1型Nef/p21激活激酶2复合物的重组与分子分析。

Reconstitution and molecular analysis of an active human immunodeficiency virus type 1 Nef/p21-activated kinase 2 complex.

作者信息

Raney Alexa, Kuo Lillian S, Baugh Laura L, Foster John L, Garcia J Victor

机构信息

Department of Internal Medicine, Division of Infectious Diseases, University of Texas Southwestern Medical Center at Dallas, 75390-9113, USA.

出版信息

J Virol. 2005 Oct;79(20):12732-41. doi: 10.1128/JVI.79.20.12732-12741.2005.

Abstract

Human immunodeficiency virus type 1 (HIV-1) Nef activation of p21-activated kinase 2 (PAK-2) was recapitulated in a cell-free system consisting of in vitro-transcribed RNA, rabbit reticulocyte lysate, and microsomal membranes on the basis of the following observations: (i) Nef associated with a kinase endogenous to the rabbit reticulocyte lysate that was identified as PAK-2, (ii) Nef-associated kinase activity was detected with Nefs from HIV-1(SF2), HIV-1(YU2), and SIV(mac239), (iii) kinase activation was not detected with a myristoylation-defective Nef (HIV-1(SF2)NefG2A) or with a Nef defective in PAK-2 activation but fully competent in other Nef functions (HIV-1(SF2)NefF195I), and (iv) Nef-associated kinase activation required activated endogenous p21 GTPases (Rac1 or Cdc42). The cell-free system was used to analyze the mechanism of Nef activation of PAK-2. First, studies suggest that the p21 GTPases may act transiently to enhance Nef activation of PAK-2 in vitro. Second, addition of wortmannin to the cell-free system demonstrated that Nef activation of PAK-2 does not require PI 3-kinase activity. Third, ultracentrifugation analysis revealed that whereas the majority of Nef and PAK-2 partitioned to the supernatant, Nef-associated PAK-2 activity partitioned to the membrane-containing pellet as a low-abundance complex. Lastly, Nef activation of PAK-2 in vitro requires addition of microsomal membranes either during or after translation of the Nef RNA. These results are consistent with a model in which activation of PAK-2 by Nef occurs by recruiting PAK-2 to membranes. As demonstrated herein, the cell-free system is a new and important tool in the investigation of the mechanism of PAK-2 activation by Nef.

摘要

基于以下观察结果,在由体外转录RNA、兔网织红细胞裂解物和微粒体膜组成的无细胞系统中再现了人类免疫缺陷病毒1型(HIV-1)Nef对p21激活激酶2(PAK-2)的激活作用:(i)Nef与兔网织红细胞裂解物中的一种内源性激酶相关,该激酶被鉴定为PAK-2;(ii)用来自HIV-1(SF2)、HIV-1(YU2)和猴免疫缺陷病毒(SIV)(mac239)的Nef检测到Nef相关激酶活性;(iii)用肉豆蔻酰化缺陷型Nef(HIV-1(SF2)NefG2A)或在PAK-2激活方面有缺陷但在其他Nef功能方面完全正常的Nef(HIV-1(SF2)NefF195I)未检测到激酶激活;(iv)Nef相关激酶激活需要激活的内源性p21 GTP酶(Rac1或Cdc42)。该无细胞系统用于分析Nef激活PAK-2的机制。首先,研究表明p21 GTP酶可能短暂起作用以增强体外Nef对PAK-2的激活。其次,向无细胞系统中添加渥曼青霉素表明Nef激活PAK-2不需要PI 3激酶活性。第三,超速离心分析显示,虽然大多数Nef和PAK-2分配到上清液中,但Nef相关的PAK-2活性作为一种低丰度复合物分配到含膜沉淀中。最后,体外Nef激活PAK-2需要在Nef RNA翻译期间或之后添加微粒体膜。这些结果与一个模型一致。在该模型中,Nef通过将PAK-2募集到膜上来激活PAK-2。如本文所示,该无细胞系统是研究Nef激活PAK-2机制的一种新的重要工具。

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