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Expression of the major glycoprotein G of human respiratory syncytial virus from recombinant vaccinia virus vectors.

机译:从重组牛痘病毒载体表达人呼吸道合胞病毒的主要糖蛋白G。

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摘要

The major glycoprotein, G, of human respiratory syncytial (RS) virus is a Mr 84,000-90,000 species that has about 60% of its mass contributed by carbohydrate, most of which is in the form of O-linked oligosaccharides. The G protein contains neither a hydrophobic N-terminal signal sequence nor a hydrophobic C-terminal anchor region. Instead, its amino acid sequence reveals only one region with significant hydrophobic character, which is between residues 38 and 66. In order to study the synthesis, processing, and functions of this unusual viral glycoprotein, full-length cDNA copies of the G protein mRNA were inserted into the DNA genome of vaccinia virus (VV) in a position that was adjacent to a strong VV promoter and within the VV gene for thymidine kinase (TK). The resulting TK- recombinant viruses were selected, plaque-purified, and characterized by Southern blot analysis of restriction enzyme digests of the viral DNA. Recombinant RNA transcripts that contained both G-specific and VV-specific sequences accumulated in cells infected with recombinant viruses having the G protein gene in the positive orientation. The translation product of these transcripts in infected cells was a Mr 84,000-90,000 glycoprotein that was indistinguishable from authentic RS virus G protein. It could be detected in cell lysates after metabolic labeling with [3H]glucosamine and was immunoprecipitated by anti-RS-virus antiserum. Immunofluorescence studies showed that the G protein accumulated intracellularly with the perinuclear distribution that is characteristic of newly synthesized glycoproteins. Furthermore, the protein was also clearly detectable on the surface of recombinant-infected cells, showing that it was transported to and inserted into the plasma membrane.
机译:人类呼吸道合胞(RS)病毒的主要糖蛋白G是一种84,000-90,000先生种,其质量中约60%由碳水化合物贡献,其中大部分为O-连接寡糖形式。 G蛋白既不包含疏水性N末端信号序列,也不包含疏水性C末端锚定区。取而代之的是,其氨基酸序列仅揭示了一个具有显着疏水特性的区域,位于残基38和66之间。为了研究这种不寻常的病毒糖蛋白的合成,加工和功能,G蛋白mRNA的全长cDNA拷贝将其插入到牛痘病毒(VV)的DNA基因组中,该基因组与强VV启动子相邻且在胸苷激酶(TK)的VV基因内。选择所得的TK重组病毒,空斑纯化,并通过病毒DNA的限制性酶消化的Southern印迹分析来表征。重组RNA转录本包含G特异性和VV特异性序列,这些序列在感染了具有正向G蛋白基因的重组病毒的细胞中积累。这些转录本在感染细胞中的翻译产物是Mr 84,000-90,000糖蛋白,与真正的RS病毒G蛋白没有区别。用[3H]葡糖胺进行代谢标记后,可在细胞裂解物中检测到它,并通过抗RS病毒抗血清免疫沉淀。免疫荧光研究表明,G蛋白在细胞内积累,具有核周分布,这是新合成糖蛋白的特征。此外,还可以在重组感染细胞的表面上清楚地检测到该蛋白质,表明该蛋白质已被运输到质膜并插入质膜。

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