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HIV-1 Gag的N端基质结构域足以通过膜靶向机制介导病毒蛋白U增强颗粒释放,但并非必需。

The N-terminal matrix domain of HIV-1 Gag is sufficient but not necessary for viral protein U-mediated enhancement of particle release through a membrane-targeting mechanism.

作者信息

Deora A, Spearman P, Ratner L

机构信息

Department of Medicine, Washington University School of Medicine, St. Louis, Missouri, 63110, USA.

出版信息

Virology. 2000 Apr 10;269(2):305-12. doi: 10.1006/viro.1999.0094.

Abstract

Viral protein U (Vpu) is an 81 amino acid phosphoprotein found in human immunodeficiency virus type 1 (HIV-1)-infected cells. One function of Vpu is to enhance the release of virus particles from the plasma membrane in infected cells. Using subcellular fractionation, we observed that Vpu promotes the targeting of Pr55 Gag to the plasma membrane, the site of viral assembly. Deletions of Pr55, which removed most of the N-terminal matrix domain (p39) or the C-terminal domains of nucleocapsid and p6 (p41), still allowed for virus-like particle production. Moreover, the release of these particles remained Vpu-responsive. The N-terminal matrix (MA) domain of Gag, which contains its membrane-binding domain, is sufficient for Vpu-mediated enhanced release into the supernatant. Furthermore, a MA-GFP fusion protein showed enhanced membrane binding in the presence of Vpu. This demonstrates that Vpu action may be mediated by allowing Gag, specifically the N-terminal matrix domain, to efficiently associate with the plasma membrane. Thus MA appears sufficient but not necessary for Vpu-mediated enhanced particle release.

摘要

病毒蛋白U(Vpu)是一种在1型人类免疫缺陷病毒(HIV-1)感染细胞中发现的含81个氨基酸的磷蛋白。Vpu的一个功能是增强感染细胞中病毒颗粒从质膜的释放。通过亚细胞分级分离,我们观察到Vpu促进Pr55 Gag靶向质膜,即病毒组装的部位。删除Pr55中去除大部分N端基质结构域(p39)或核衣壳和p6的C端结构域(p41)的部分,仍能产生病毒样颗粒。此外,这些颗粒的释放仍对Vpu有反应。Gag的N端基质(MA)结构域包含其膜结合结构域,足以实现Vpu介导的向上清液中增强释放。此外,一种MA-GFP融合蛋白在有Vpu存在时显示出增强的膜结合。这表明Vpu的作用可能是通过使Gag,特别是N端基质结构域,有效地与质膜结合来介导的。因此,MA对于Vpu介导的颗粒释放增强似乎是足够的,但不是必需的。

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