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Virus-receptor interaction in the adenovirus system I. Identification of virion attachment proteins of the HeLa cell plasma membrane.

机译:腺病毒系统中的病毒-受体相互作用I. HeLa细胞质膜病毒体附着蛋白的鉴定。

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摘要

Plasma membranes from HeLa cells were isolated in a two-phase polymer system. To compare the efficiency of attachment protein extraction, a normalized assay for the assessment of adenovirus type 2 (Ad2) receptor-active components interfering with the attachment of Ad2 to HeLa cells was developed. An optimized detergent extraction procedure, 0.5% Triton X-100, was used, and solubilized membrane proteins were radioisotope labeled in vitro. Proteins with affinity for Ad2 virions were quantified and identified in a sucrose gradient sedimentation assay and by affinity chromatography with cross-linked Ad2 virions immobilized to AH-Sepharose 4B. From virions recovered in the sucrose gradient system, one major membrane component of high affinity was identified with a polypeptide molecular weight of around 40,000. Glycosylated proteins isolated by wheat germ lectin chromatography with high affinity for immobilized virus particles were isolated, and two major components with apparent molecular weights of 40,000 and 42,000 were identified. We suggest that a glycosylated protein with high affinity for Ad2 virions and a polypeptide molecular weight of 40,000 to 42,000 is one component of the Ad2 attachment site on HeLa cells.
机译:在两相聚合物系统中分离了HeLa细胞的质膜。为了比较附着蛋白提取的效率,开发了一种标准化的测定方法,用于评估2型腺病毒(Ad2)受体活性成分干扰Ad2与HeLa细胞的附着。使用了最优化的去污剂提取程序,即0.5%Triton X-100,并在体外用放射性同位素标记了溶解的膜蛋白。对具有对Ad2病毒体的亲和力的蛋白质进行定量,并在蔗糖梯度沉降测定中进行鉴定,并通过亲和层析,将交联的Ad2病毒体固定在AH-Sepharose 4B上。从在蔗糖梯度系统中回收的病毒体中,鉴定出一种高亲和力的主要膜组分,其多肽分子量约为40,000。分离了通过小麦胚凝集素色谱分离的糖基化蛋白,该蛋白对固定化病毒颗粒具有高亲和力,并鉴定了两个主要成分,其表观分子量分别为40,000和42,000。我们建议对Ad2病毒体具有高亲和力且多肽分子量为40,000至42,000的糖基化蛋白是HeLa细胞上Ad2附着位点的一个组成部分。

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