FRET-Based Detection and Quantification of HIV-1 Virion Maturation

被引:4
|
作者
Sarca, Anamaria D. [1 ]
Sardo, Luca [2 ,4 ]
Fukuda, Hirofumi [1 ]
Matsui, Hiroyuki [1 ]
Shirakawa, Kotaro [1 ]
Horikawa, Kazuki [3 ]
Takaori-Kondo, Akifumi [1 ]
Izumi, Taisuke [1 ,5 ]
机构
[1] Kyoto Univ, Grad Sch Med, Dept Hematol & Oncol, Kyoto, Japan
[2] Univ Sci, Dept Biol Sci, Philadelphia, PA USA
[3] Tokushima Univ, Adv Res Promot Ctr, Dept Opt Imaging, Tokushima, Japan
[4] Merck & Co Inc, MRL, Dept Infect Dis & Vaccines, West Point, PA USA
[5] Walter Reed Army Inst Res, Henry M Jackson Fdn Adv, Mil Med Inc, Support Mil HIV Res Program, Silver Spring, MD 20910 USA
来源
FRONTIERS IN MICROBIOLOGY | 2021年 / 12卷
基金
日本学术振兴会;
关键词
HIV-1 Gag maturation; Fö rster Resonance Energy Transfer; single virion imaging; protease inhibitor; fluorescence microscopy;
D O I
10.3389/fmicb.2021.647452
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
HIV-1 infectivity is achieved through virion maturation. Virus particles undergo structural changes via cleavage of the Gag polyprotein mediated by the viral protease, causing the transition from an uninfectious to an infectious status. The majority of proviruses in people living with HIV-1 treated with combination antiretroviral therapy are defective with large internal deletions. Defective proviral DNA frequently preserves intact sequences capable of expressing viral structural proteins to form virus-like particles whose maturation status is an important factor for chronic antigen-mediated immune stimulation and inflammation. Thus, novel methods to study the maturation capability of defective virus particles are needed to characterize their immunogenicity. To build a quantitative tool to study virion maturation in vitro, we developed a novel single virion visualization technique based on fluorescence resonance energy transfer (FRET). We inserted an optimized intramolecular CFP-YPF FRET donor-acceptor pair bridged with an HIV-1 protease cleavage sequence between the Gag MA-CA domains. This system allowed us to microscopically distinguish mature and immature virions via their FRET signal when the FRET donor and acceptor proteins were separated by the viral protease during maturation. We found that approximately 80% of the FRET labeled virus particles were mature with equivalent infectivity to wild type. The proportion of immature virions was increased by treatment of virus producer cells with a protease inhibitor in a dose-dependent manner, which corresponded to a relative decrease in infectivity. Potential areas of application for this tool are assessing maturation efficiency in different cell type settings of intact or deficient proviral DNA integrated cells. We believe that this FRET-based single-virion imaging platform will facilitate estimating the impact on the immune system of both extracellular intact and defective viruses by quantifying the Gag maturation status.
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页数:13
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