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从非洲绿猴肾细胞中纯化白喉毒素受体

Purification of diphtheria toxin receptor from Vero cells.

作者信息

Mekada E, Senoh H, Iwamoto R, Okada Y, Uchida T

机构信息

Institute of Life Science, Kurume University, Fukuoka, Japan.

出版信息

J Biol Chem. 1991 Oct 25;266(30):20457-62.

PMID:1939100
Abstract

Diphtheria toxin receptor has been solubilized from Vero cell membranes with octyl beta-D-glucoside. CRM197, the product of a mutated diphtheria toxin gene, was used for the identification of the receptor. The binding activity of the solubilized receptor was assayed by precipitating the receptor with acetone in the presence of phospholipids and carrier proteins. The solubilized receptor was purified by the combination of several chromatographic steps in the presence of the detergent, resulting in about a 10(6)-fold purification of the receptor. The purified receptor showed essentially a single band of 14.5 kDa by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. When partially purified receptor fractions were subjected to ligand blotting analysis using 125I-CRM197 as the probe, the 14.5-kDa protein and a few minor protein bands were identified as diphtheria toxin-binding molecules. These results show clearly that the 14.5-kDa protein is the diphtheria toxin receptor, or at least the major diphtheria toxin-binding molecule. When partially purified receptor was applied to a Sephacryl S-300 column in the presence of detergent, the receptor was eluted in the fractions corresponding to the 60-90-kDa size range. This suggests that the protein forms a complex with itself or with another protein.

摘要

已用辛基-β-D-葡萄糖苷从非洲绿猴肾细胞(Vero细胞)膜中溶解出白喉毒素受体。使用突变的白喉毒素基因产物CRM197来鉴定该受体。通过在磷脂和载体蛋白存在的情况下用丙酮沉淀受体来测定溶解受体的结合活性。在去污剂存在的情况下,通过几个色谱步骤的组合对溶解的受体进行纯化,使受体纯化了约10^6倍。经十二烷基硫酸钠-聚丙烯酰胺凝胶电泳分析,纯化后的受体在14.5 kDa处基本呈现单一条带。当使用125I-CRM197作为探针,对部分纯化的受体组分进行配体印迹分析时,14.5 kDa的蛋白质和一些次要蛋白条带被鉴定为白喉毒素结合分子。这些结果清楚地表明,14.5 kDa的蛋白质是白喉毒素受体,或者至少是主要的白喉毒素结合分子。当在去污剂存在的情况下,将部分纯化的受体应用于Sephacryl S-300柱时,受体在对应于60 - 90 kDa大小范围的组分中被洗脱。这表明该蛋白质与自身或与另一种蛋白质形成复合物。

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