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牛神经垂体分泌囊泡的分离与鉴定

Isolation and characterization of secretory vesicles from bovine neurohypophyses.

作者信息

Gratzl M, Torp-Pedersen C, Dartt D, Treiman M, Thorn N A

出版信息

Hoppe Seylers Z Physiol Chem. 1980 Nov;361(11):1615-28. doi: 10.1515/bchm2.1980.361.2.1615.

Abstract

A procedure is described for the isolation of secretory vesicles from bovine neurohypophyses by differential centrifugation followed by density gradient centrifugation on iso-osmolal gradients of percoll/sucrose. Only negligible contamination of the secretory vesicle fraction with markers for mitochondria, microsomes and plasma membranes could be detected. The amount of Ca2-ATPase in the isolated neurohypophysial secretory vesicles was of the same low order of magnitude as that of (Na, K)-ATPase. Thin-section electromicrographs confirmed the high purity of the isolated secretory vesicle fractions, In freeze-fracture electronmicrographs, vesicle fusion was demonstrated after incubation with Ca2. As shown in dodecyl sulfate-gel electrophoresis and subsequent autoradiography secretory vesicles exhibited an endogenous phosphorylation activity. The secretory vesicles contained an average of 23.1 microgram vasopressin/mg of protein. On incubation in media differing in ionic strength, pH and Ca2 concentration the vesicles were stable for at least 1 h.

摘要

本文描述了一种从牛神经垂体中分离分泌囊泡的方法,先通过差速离心,然后在等渗的 Percoll/蔗糖密度梯度上进行密度梯度离心。仅检测到分泌囊泡部分被线粒体、微粒体和质膜标记物的污染可忽略不计。分离的神经垂体分泌囊泡中 Ca2-ATP 酶的量与 (Na, K)-ATP 酶的量处于相同的低数量级。超薄切片电子显微镜照片证实了分离的分泌囊泡部分的高纯度,在冷冻断裂电子显微镜照片中,与 Ca2 孵育后显示出囊泡融合。如十二烷基硫酸钠凝胶电泳及随后的放射自显影所示,分泌囊泡表现出内源性磷酸化活性。分泌囊泡平均含有 23.1 微克加压素/毫克蛋白质。在离子强度、pH 和 Ca2 浓度不同的培养基中孵育时,囊泡至少稳定 1 小时。

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