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麻疹病毒融合蛋白在参与细胞融合的跨膜-胞质内半胱氨酸残基上发生棕榈酰化。

Measles virus fusion protein is palmitoylated on transmembrane-intracytoplasmic cysteine residues which participate in cell fusion.

作者信息

Caballero M, Carabaña J, Ortego J, Fernández-Muñoz R, Celma M L

机构信息

Molecular Virology Laboratory, Hospital "Ramón y Cajal" Instituto Nacional de la Salud, Madrid 28034, Spain.

出版信息

J Virol. 1998 Oct;72(10):8198-204. doi: 10.1128/JVI.72.10.8198-8204.1998.

Abstract

[3H]palmitic acid was metabolically incorporated into the viral fusion protein (F) of Edmonston or freshly isolated measles virus (MV) during infection of human lymphoid or Vero cells. The uncleaved precursor F0 and the F1 subunit from infected cells and extracellular virus were both labeled, indicating that palmitoylation can take place prior to F0 cleavage and that palmitoylated F protein was incorporated into virus particles. [3H]palmitic acid was released from F protein upon hydroxylamine or dithiothreitol treatment, indicating a thioester linkage. In cells transfected with the cloned MV F gene, in which the cysteines located in the intracytoplasmic and transmembrane domains (Cys 506, 518, 519, 520, and 524) were replaced by serine, a major reduction of [3H]palmitic acid incorporation was observed for F mutated at Cys 506 and, to a lesser extent, at Cys 518 and Cys 524. We also observed incorporation of [3H]palmitic acid in the F1 subunit of canine distemper virus F protein. Cell fusion induced by cotransfection of cells with MV F and H (hemagglutinin) genes was significantly reduced after replacement of Cys 506 or Cys 519 with serine in the MV F gene. Transfection with the F gene with a mutation for Cys 518 abolished cell fusion, although less mutant protein was detected on the cell surface. These results suggest that the F protein transmembrane domain cysteines 506 and 518 participate in structures involved in cell fusion, possibly mediated by palmitoylation.

摘要

在人淋巴细胞或非洲绿猴肾细胞(Vero细胞)感染期间,[3H]棕榈酸通过代谢作用掺入埃德蒙斯顿麻疹病毒(MV)或新分离的麻疹病毒的病毒融合蛋白(F)中。来自受感染细胞和细胞外病毒的未切割前体F0和F1亚基均被标记,这表明棕榈酰化可在F0切割之前发生,并且棕榈酰化的F蛋白被掺入病毒颗粒中。用羟胺或二硫苏糖醇处理后,[3H]棕榈酸从F蛋白中释放出来,表明存在硫酯键。在用克隆的MV F基因转染的细胞中,位于胞质内和跨膜结构域的半胱氨酸(Cys 506、518、519、520和524)被丝氨酸取代,在Cys 506处发生突变的F蛋白中观察到[3H]棕榈酸掺入量大幅减少,在Cys 518和Cys 524处发生突变的F蛋白中[3H]棕榈酸掺入量也有一定程度的减少。我们还观察到[3H]棕榈酸掺入犬瘟热病毒F蛋白的F1亚基中。在MV F基因中用丝氨酸取代Cys 506或Cys 519后,与MV F和血凝素(H)基因共转染细胞诱导的细胞融合显著降低。用Cys 518发生突变的F基因转染可消除细胞融合,尽管在细胞表面检测到的突变蛋白较少。这些结果表明,F蛋白跨膜结构域的半胱氨酸506和518参与了细胞融合相关结构,可能是由棕榈酰化介导的。

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