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棕榈酰辅酶A和肉豆蔻酰辅酶A的生物正交模拟物,以及它们随后通过点击化学进行的分离和通过质谱进行的表征,揭示了由HIV-1感染修饰的新型酰化宿主蛋白。

Bioorthogonal mimetics of palmitoyl-CoA and myristoyl-CoA and their subsequent isolation by click chemistry and characterization by mass spectrometry reveal novel acylated host-proteins modified by HIV-1 infection.

作者信息

Colquhoun David R, Lyashkov Alexey E, Ubaida Mohien Ceereena, Aquino Veronica N, Bullock Brandon T, Dinglasan Rhoel R, Agnew Brian J, Graham David R M

机构信息

Department of Molecular and Comparative Pathobiology, Johns Hopkins University School of Medicine, Baltimore, MD, USA.

W. Harry Feinstone Department of Molecular Microbiology and Immunology, Johns Hopkins Bloomberg School of Public Health, Baltimore, MD, USA.

出版信息

Proteomics. 2015 Jun;15(12):2066-77. doi: 10.1002/pmic.201500063. Epub 2015 May 26.

DOI:10.1002/pmic.201500063
PMID:25914232
Abstract

Protein acylation plays a critical role in protein localization and function. Acylation is essential for human immunodeficiency virus 1 (HIV-1) assembly and budding of HIV-1 from the plasma membrane in lipid raft microdomains and is mediated by myristoylation of the Gag polyprotein and the copackaging of the envelope protein is facilitated by colocalization mediated by palmitoylation. Since the viral accessory protein NEF has been shown to alter the substrate specificity of myristoyl transferases, and alter cargo trafficking lipid rafts, we hypothesized that HIV-1 infection may alter protein acylation globally. To test this hypothesis, we labeled HIV-1 infected cells with biomimetics of acyl azides, which are incorporated in a manner analogous to natural acyl-Co-A. A terminal azide group allowed us to use a copper catalyzed click chemistry to conjugate the incorporated modifications to a number of substrates to carry out SDS-PAGE, fluorescence microscopy, and enrichment for LC-MS/MS. Using LC-MS/MS, we identified 103 and 174 proteins from the myristic and palmitic azide enrichments, with 27 and 45 proteins respectively that differentiated HIV-1 infected from uninfected cells. This approach has provided us with important insights into HIV-1 biology and is widely applicable to many virological systems.

摘要

蛋白质酰化在蛋白质定位和功能中起着关键作用。酰化对于人类免疫缺陷病毒1型(HIV-1)的组装以及HIV-1从脂筏微结构域中的质膜出芽至关重要,它由Gag多蛋白的肉豆蔻酰化介导,包膜蛋白的共包装则通过棕榈酰化介导的共定位得以促进。由于病毒辅助蛋白NEF已被证明会改变肉豆蔻酰转移酶的底物特异性,并改变货物在脂筏中的运输,我们推测HIV-1感染可能会在整体上改变蛋白质酰化。为了验证这一假设,我们用酰基叠氮化物的仿生类似物标记HIV-1感染的细胞,这些类似物以类似于天然酰基辅酶A的方式被掺入。末端叠氮基团使我们能够利用铜催化的点击化学将掺入的修饰与多种底物偶联,以进行SDS-PAGE、荧光显微镜检查以及用于LC-MS/MS的富集。使用LC-MS/MS,我们从肉豆蔻酰叠氮化物和棕榈酰叠氮化物富集物中分别鉴定出103种和174种蛋白质,其中分别有27种和45种蛋白质能够区分HIV-1感染细胞和未感染细胞。这种方法为我们深入了解HIV-1生物学提供了重要见解,并且广泛适用于许多病毒学系统。

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