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Analyses of disulfides present in the rubella virus E1 glycoprotein

机译:风疹病毒E1糖蛋白中二硫化物的分析

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The surface of Rubella virus contains the glycoproteins E1 and E2. The E1 protein induces neutralizing antibodies and has been implicated in the process of recognition of cellular receptors. To gain information on the structural organization of the E1 protein we have analyzed the disulfide bonds present within this molecule. The reactivity of the protein with radioactively labeled iodoacetic acid indicates that all 20 cysteine residues present in the ectodomain of the E1 protein are involved in disulfide formation. E1 protein was purified by preparative SDS-PAGE under nonreducing conditions from virus particles grown in tissue culture in the presence of [35S]cysteine. The purified protein was digested with a number of proteases followed by reversed phase high-performance liquid chromatography (HPLC). [35S]cysteine-containing peptides were identified and characterized by N-terminal amino acid sequence determination. These analyses identified the following eight disulfide bridges: C(1)-C(2); C(3)-C(15); C(6)-C(7); C(9)-C(10); C(11)-C(12); C(13)-C(14); C(17)-C(18); and C(19)-C(20). The two disulfide bridges formed by the residues C(4), C(5), C(8), and C(16) have not been identified with certainty, but a likely organization can be derived. The data obtained are discussed in the context of a possible structural and functional organization of the E1 protein.
机译:风疹病毒的表面含有糖蛋白E1和E2。 E1蛋白诱导中和抗体,并已参与细胞受体的识别过程。为了获得有关E1蛋白的结构组织的信息,我们分析了该分子内存在的二硫键。该蛋白质与放射性标记的碘乙酸的反应性表明,存在于E1蛋白质胞外域的所有20个半胱氨酸残基均参与二硫键的形成。在非还原条件下,通过制备SDS-PAGE从[35S]半胱氨酸存在下在组织培养中生长的病毒颗粒中纯化E1蛋白。纯化的蛋白质用多种蛋白酶消化,然后进行反相高效液相色谱(HPLC)消化。鉴定并通过N端氨基酸序列确定来鉴定含有[35S]半胱氨酸的肽。这些分析确定了以下八个二硫键:C(1)-C(2); C(3)-C(15); C(6)-C(7); C(9)-C(10); C(11)-C(12); C(13)-C(14); C(17)-C(18);和C(19)-C(20)。尚不能确定由残基C(4),C(5),C(8)和C(16)形成的两个二硫键,但可以推导出可能的结构。在E1蛋白可能的结构和功能组织的背景下讨论了获得的数据。

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