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参与核糖体结合的肝细胞膜蛋白:通过三种方法进行鉴定。

Hepatic membrane proteins involved in ribosome binding: identification by three procedures.

作者信息

Aulinskas T H, Burden T S

出版信息

Hoppe Seylers Z Physiol Chem. 1979 Jun;360(6):709-20. doi: 10.1515/bchm2.1979.360.1.709.

Abstract

Rat liver ribosomes, isolated from rough-surfaced endoplasmic reticulum using non-ionic detergent in the presence of 25 mM KCl, were associated with non-ribosomal proteins, presumably of membranous origin. These proteins could be isolated by extracting such ribosome fractions with either deoxycholate or non-ionic detergents at higher concentrations of KCl. Analysis of the extracts by polyacrylamide gel electrophoresis in the presence of sodium dodecyl sulphate revealed the presence of a number of discrete polypeptides having the following approximate molecular weights: 166,000, 107,000, 100,000, 65,000 and 36,000. Ribosomes associated with the membrane-derived proteins reattached to degranulated membranes in vitro less well than did ribosomes prepared in ways which removed the proteins. Extraction of a set of similar proteins from degranulated endoplasmic reticulum by treatment with buffered 1 M urea, also interfered with ribosome reattachment. A third approach to the identification of proteins associated with ribosome attachment sites involved the labelling with radioactive succinic anhydride of apparently similar proteins in degranulated membranes, after prior treatment of the latter, before removal of bound ribosomes, with unlabelled reagent. The results indicate that certain membrane proteins may be part of the receptor sites for binding of ribosomes to the endoplasmic reticulum in rat liver.

摘要

用非离子去污剂在25 mM氯化钾存在的条件下从糙面内质网分离得到的大鼠肝脏核糖体,与可能来源于膜的非核糖体蛋白相关联。这些蛋白质可以通过在较高浓度的氯化钾条件下用脱氧胆酸盐或非离子去污剂提取此类核糖体组分来分离。在十二烷基硫酸钠存在的条件下通过聚丙烯酰胺凝胶电泳对提取物进行分析,结果显示存在一些具有以下近似分子量的离散多肽:166,000、107,000、100,000、65,000和36,000。与膜衍生蛋白相关联的核糖体在体外重新附着到脱粒膜上的效果不如以去除这些蛋白的方式制备的核糖体。用缓冲的1 M尿素处理从脱粒内质网中提取一组类似的蛋白质,也会干扰核糖体的重新附着。鉴定与核糖体附着位点相关的蛋白质的第三种方法涉及在去除结合的核糖体之前,先用未标记的试剂处理脱粒膜,然后用放射性琥珀酸酐标记其中明显类似的蛋白质。结果表明,某些膜蛋白可能是大鼠肝脏中核糖体与内质网结合的受体位点的一部分。

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