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Effects of disulfide bridges glycoprotein E1 on fusogenic activity of Rubella virus.

机译:二硫键糖蛋白E1对风疹病毒融合活性的影响。

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Rubella virus (RUBV) infects cells via an acid-triggered membrane fusion process. RUBV virions contain two cysteine-rich glycoproteins, E2 and E1. The latter is believed to be involved in the membrane fusion. Using a recombinant plasmid containing RUBV E1 and E2, 11 of total 20 cysteines present in the ectodomain of wild type E1 were mutated to test their role in the fusion via the formation of disulfide bridges. The recombinant plasmids containing mutated E1 (Cys2-Cys20) or wild type (wt) E1 were expressed in BHK-21 cells. Their fusogenic and hemadsorption activities in addition to a potential of cell surface expression of E1 and E2 were assayed. The results showed that the fusogenic activity was lost in all tested mutants, while the hemadsorption activity and cell surface expression potential were affected differently in individual mutants. Since only the Cys5 and Cys8 mutations led to a reduction of both hemadsorption and cell surface expression, we assume that these mutations prevented the formation of the disulfide bridge, what led to a misfolding of E1 and consequently to a failure of recognition of E1 by E2. In conclusion, the disulfide bridges disrupted in all the tested mutants appear essential for the cell fusion, while only the disulfide bridge C(5)-C(8) seems to be crucial for the transport of E1 and E2 in the cell.
机译:风疹病毒(RUBV)通过酸触发的膜融合过程感染细胞。 RUBV病毒体包含两个富含半胱氨酸的糖蛋白,E2和E1。后者被认为与膜融合有关。使用包含RUBV E1和E2的重组质粒,将野生型E1胞外域中存在的总共20个半胱氨酸中的11个半胱氨酸突变,以通过形成二硫键测试它们在融合中的作用。含有突变的E1(Cys2-Cys20)或野生型(wt)E1的重组质粒在BHK-21细胞中表达。除了潜在的E1和E2细胞表面表达外,还测定了它们的融合和溶血活性。结果表明,在所有测试的突变体中融合活性都丧失了,而单个突变体的吸血活性和细胞表面表达潜力受到不同的影响。由于仅Cys5和Cys8突变会导致血液吸附和细胞表面表达的降低,因此我们假设这些突变阻止了二硫键的形成,这导致E1错折叠并因此导致E2无法识别E1。 。总之,在所有测试的突变体中破坏的二硫键似乎是细胞融合所必需的,而只有二硫键C(5)-C(8)似乎对细胞中E1和E2的运输至关重要。

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