Kotov A, Zhou J, Flicker P, Aiken C
Department of Microbiology and Immunology, Vanderbilt University School of Medicine, Nashville, Tennessee, USA.
J Virol. 1999 Oct;73(10):8824-30. doi: 10.1128/JVI.73.10.8824-8830.1999.
Highly conserved among primate lentiviruses, the human immunodeficiency virus type 1 (HIV-1) Nef protein enhances viral infectivity by an unknown mechanism. Nef-defective virions are blocked at a stage of the HIV-1 life cycle between entry and reverse transcription, possibly virus uncoating. Nef is present in purified HIV-1 particles; however, it has not been determined whether Nef is specifically recruited into HIV-1 particles or whether virion-associated Nef plays a functional role in HIV-1 replication. To address the specificity and potential functionality of virion-associated Nef, we determined the subviral localization of Nef. HIV-1 cores were isolated by detergent treatment of concentrated virions followed by equilibrium density gradient sedimentation. Relative to HIV-1 virions, HIV-1 cores contained equivalent amounts of reverse transcriptase and integrase, decreased amounts of the viral matrix protein, and trace quantities of the viral transmembrane glycoprotein gp41. Examination of the particles by electron microscopy revealed cone-shaped structures characteristic of lentiviral cores. Similar quantities of proteolytically processed Nef protein were detected in gradient fractions of HIV-1 cores and intact virions. In addition, detergent-resistant subviral complexes isolated from immature HIV-1 particles contained similar quantities of Nef as untreated virions. These results demonstrate that Nef stably associates with the HIV-1 core and suggest that virion-associated Nef plays a functional role in accelerating HIV-1 replication.
人类免疫缺陷病毒1型(HIV-1)的Nef蛋白在灵长类慢病毒中高度保守,其通过未知机制增强病毒感染性。Nef缺陷型病毒粒子在HIV-1生命周期中进入与逆转录之间的阶段受阻,可能是病毒脱壳阶段。Nef存在于纯化的HIV-1颗粒中;然而,尚未确定Nef是否被特异性招募到HIV-1颗粒中,或者病毒体相关的Nef在HIV-1复制中是否发挥功能作用。为了研究病毒体相关Nef的特异性和潜在功能,我们确定了Nef的亚病毒定位。通过对浓缩病毒粒子进行去污剂处理,然后进行平衡密度梯度沉降来分离HIV-1核心。相对于HIV-1病毒粒子,HIV-1核心含有等量的逆转录酶和整合酶,病毒基质蛋白的量减少,以及痕量的病毒跨膜糖蛋白gp41。通过电子显微镜检查颗粒发现了慢病毒核心特有的锥形结构。在HIV-1核心和完整病毒粒子的梯度级分中检测到相似量的经蛋白水解处理的Nef蛋白。此外,从不成熟HIV-1颗粒中分离出的抗去污剂亚病毒复合物含有与未处理病毒粒子相似量的Nef。这些结果表明Nef与HIV-1核心稳定结合,并表明病毒体相关的Nef在加速HIV-1复制中发挥功能作用。