Kinetics of HIV-1 capsid uncoating revealed by single-molecule analysis

被引:78
|
作者
Marquez, Chantal L. [1 ,2 ]
Lau, Derrick [1 ,2 ]
Walsh, James [1 ,2 ]
Shah, Vaibhav [1 ,2 ]
McGuinness, Conall [1 ,2 ]
Wong, Andrew [3 ]
Aggarwal, Anupriya [3 ]
Parker, Michael W. [4 ,5 ]
Jacques, David A. [1 ]
Turville, Stuart [3 ]
Bocking, Till [1 ,2 ]
机构
[1] UNSW, Sch Med Sci, EMBL Australia Node Single Mol Sci, Sydney, NSW, Australia
[2] UNSW, ARC Ctr Excellence Adv Mol Imaging, Sydney, NSW, Australia
[3] Kirby Inst, Sydney, NSW, Australia
[4] St Vincent s Inst Med Res, Rational Drug Discovery Ctr, Australian Canc Res Fdn, Melbourne, Vic, Australia
[5] Univ Melbourne, Mol Sci & Biotechnol Inst Bio21, Dept Biochem & Mol Biol, Melbourne, Vic, Australia
来源
ELIFE | 2018年 / 7卷
基金
英国医学研究理事会;
关键词
VIRUS; RECOGNITION; CYCLOPHILIN; CORE; RECONSTRUCTIONS; STABILIZATION; MATURATION; MECHANISM; CYTOLYSIN; PROTEINS;
D O I
10.7554/eLife.34772
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
Uncoating of the metastable HIV-1 capsid is a tightly regulated disassembly process required for release of the viral cDNA prior to nuclear import. To understand the intrinsic capsid disassembly pathway and how it can be modulated, we have developed a single-particle fluorescence microscopy method to follow the real-time uncoating kinetics of authentic HIV capsids in vitro immediately after permeabilizing the viral membrane. Opening of the first defect in the lattice is the rate-limiting step of uncoating, which is followed by rapid, catastrophic collapse. The capsid-binding inhibitor PF74 accelerates capsid opening but stabilizes the remaining lattice. In contrast, binding of a polyanion to a conserved arginine cluster in the lattice strongly delays initiation of uncoating but does not prevent subsequent lattice disassembly. Our observations suggest that different stages of uncoating can be controlled independently with the interplay between different capsid-binding regulators likely to determine the overall uncoating kinetics.
引用
收藏
页数:23
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