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大鼠肝脏溶酶体膜中酶和糖蛋白的特性分析。

Characterization of enzymes and glycoproteins in rat liver lysosomal membranes.

作者信息

Yamamoto K, Ikehara Y, Kawamoto S, Kato K

出版信息

J Biochem. 1980 Jan;87(1):237-48. doi: 10.1093/oxfordjournals.jbchem.a132731.

Abstract

A simple method for the preparation of lysosomes from livers of rats injected with Triton WR 1339 was developed. Enzymic characterization showed that the Triton WR 1339-filled lysosome (tritosome) preparation isolated by this procedure was almost completely free from mitochondria, peroxisomes, and microsomes. With this method, tritosomes were purified about 50 times with a yield of 8%. The tritosomal membrane fraction was prepared by osmotic disruption of the purified tritosomes followed by washing with 1 M NaCl. Analysis by SDS-polyacrylamide gel electrophoresis showed that tritosomal membrane proteins were distinct from those of plasma membranes. The major glycoproteins found in tritosomal membranes in the higher molecular weight region were not detected in plasma membranes. When livers were labeled with L-[3H]leucine or D-[3H]glucosamine, the incorporation of both isotopes into tritosomes attained the maximum value at around 3 h after the isotope injection. Radioactivities associated with the tritosomal membranes decayed slower than those of the tritosomal contents. SDS-polyacrylamide gel electrophoresis of the membranes labeled with the isotopes for various times demonstrated the distribution and variation with time of radioactivity in the protein and glycoprotein components. The results indicate that the turnover rate of the protein and glycoprotein components in the tritosomal membrane is heterogeneous.

摘要

开发了一种从注射曲拉通WR 1339的大鼠肝脏中制备溶酶体的简单方法。酶学特性表明,通过该方法分离得到的充满曲拉通WR 1339的溶酶体(三体)制剂几乎完全不含线粒体、过氧化物酶体和微粒体。用这种方法,三体被纯化了约50倍,产率为8%。通过对纯化的三体进行渗透破坏,然后用1M氯化钠洗涤,制备三体膜组分。SDS-聚丙烯酰胺凝胶电泳分析表明,三体膜蛋白与质膜蛋白不同。在高分子量区域的三体膜中发现的主要糖蛋白在质膜中未检测到。当用L-[3H]亮氨酸或D-[3H]葡萄糖胺标记肝脏时,两种同位素掺入三体的量在注射同位素后约3小时达到最大值。与三体膜相关的放射性比三体内容物的放射性衰减得慢。对用同位素标记不同时间的膜进行SDS-聚丙烯酰胺凝胶电泳,证明了蛋白质和糖蛋白组分中放射性的分布及其随时间的变化。结果表明,三体膜中蛋白质和糖蛋白组分的周转率是不均匀的。

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