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具有保守磷脂酶催化基序的痘苗病毒F13L蛋白诱导B5R包膜糖蛋白在高尔基体后囊泡中共定位。

Vaccinia virus F13L protein with a conserved phospholipase catalytic motif induces colocalization of the B5R envelope glycoprotein in post-Golgi vesicles.

作者信息

Husain M, Moss B

机构信息

Laboratory of Viral Diseases, National Institute of Allergy and Infectious Diseases, National Institutes of Health, Bethesda, Maryland 20892-0445, USA.

出版信息

J Virol. 2001 Aug;75(16):7528-42. doi: 10.1128/JVI.75.16.7528-7542.2001.

Abstract

The wrapping of intracellular mature vaccinia virions by modified trans-Golgi or endosomal cisternae to form intracellular enveloped virions is dependent on at least two viral proteins encoded by the B5R and F13L open reading frames. B5R is a type I integral membrane glycoprotein, whereas F13L is an unglycosylated, palmitylated protein with a motif that is conserved in a superfamily of phospholipid-metabolizing enzymes. Microscopic visualization of the F13L protein was achieved by fusing it to the enhanced green fluorescent protein (GFP). F13L-GFP was functional when expressed by a recombinant vaccinia virus in which it replaced the wild-type F13L gene or by transfection of uninfected cells with a plasmid vector followed by infection with an F13L deletion mutant. In uninfected or infected cells, F13L-GFP was associated with Golgi cisternae and post-Golgi vesicles containing the LAMP 2 late endosomal-lysosomal marker. Association of F13L-GFP with vesicles was dependent on an intact phospholipase catalytic motif and sites of palmitylation. The B5R protein was also associated with LAMP2-containing vesicles when F13L-GFP was coexpressed, but was largely restricted to Golgi cisternae in the absence of F13L-GFP or when the F13L moiety was mutated. We suggest that the F13L protein, like its human phospholipase D homolog, regulates vesicle formation and that this process is involved in intracellular enveloped virion membrane formation.

摘要

通过修饰的反式高尔基体或内体池对细胞内成熟痘苗病毒粒子进行包裹以形成细胞内包膜病毒粒子,这至少依赖于由B5R和F13L开放阅读框编码的两种病毒蛋白。B5R是一种I型整合膜糖蛋白,而F13L是一种未糖基化的、棕榈酰化的蛋白,其基序在磷脂代谢酶超家族中保守。通过将F13L蛋白与增强型绿色荧光蛋白(GFP)融合实现了对其的显微镜可视化。当由重组痘苗病毒表达时,F13L-GFP具有功能,其中它取代了野生型F13L基因,或者通过用质粒载体转染未感染的细胞,随后用F13L缺失突变体感染。在未感染或感染的细胞中,F13L-GFP与高尔基体池和含有LAMP 2晚期内体-溶酶体标志物的高尔基体后小泡相关联。F13L-GFP与小泡的关联依赖于完整的磷脂酶催化基序和棕榈酰化位点。当F13L-GFP共表达时,B5R蛋白也与含有LAMP2的小泡相关联,但在没有F13L-GFP或F13L部分发生突变时,B5R蛋白主要局限于高尔基体池。我们认为,F13L蛋白与其人类磷脂酶D同源物一样,调节小泡形成,并且这一过程参与细胞内包膜病毒粒子膜的形成。

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