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从大鼠肝脏匀浆中制备的高尔基体组分。I. 分离程序和形态学特征。

Golgi fractions prepared from rat liver homogenates. I. Isolation procedure and morphological characterization.

作者信息

Ehrenreich J H, Bergeron J J, Siekevitz P, Palade G E

出版信息

J Cell Biol. 1973 Oct;59(1):45-72. doi: 10.1083/jcb.59.1.45.

Abstract

In devising a new procedure for the isolation of Golgi fractions from rat liver homogenates, we have taken advantage of the overloading with very low density lipoprotein (VLDL) particles that occurs in the Golgi elements of hepatocytes approximately 90 min after ethanol is administered (0.6 g/100 g body weight) by stomach tube to the animals. The VLDLs act as morphological markers as well as density modifiers of these elements. The starting preparation is a total microsomal fraction prepared from liver homogenized (1:5) in 0.25 M sucrose. This fraction is resuspended in 1.15 M sucrose and loaded at the bottom of a discontinuous sucrose density gradient. Centrifugation at approximately 13 x 10(6)g.min yields by flotation three Golgi fractions of density >1.041 and <1.173. The light and intermediate fractions consist essentially of VLDL-loaded Golgi vacuoles and cisternae. Nearly empty, often collapsed, Golgi cisternae are the main component of the heavy fraction. A procedure which subjects the Golgi fractions to hypotonic shock and shearing in a French press at pH 8.5 allows the extraction of the content of the Golgi elements and the subsequent isolation of their membranes by differential centrifugation.

摘要

在设计一种从大鼠肝脏匀浆中分离高尔基体组分的新方法时,我们利用了在通过胃管给动物(0.6 g/100 g体重)灌胃乙醇后约90分钟,肝细胞高尔基体中出现的极低密度脂蛋白(VLDL)颗粒过载现象。VLDL既作为这些细胞器的形态学标记物,也作为其密度调节剂。起始制备物是由在0.25 M蔗糖中匀浆(1:5)的肝脏制备的总微粒体组分。该组分重悬于1.15 M蔗糖中,并加载到不连续蔗糖密度梯度的底部。以约13×10(6)g·min进行离心,通过漂浮可得到密度>1.041且<1.173的三个高尔基体组分。轻组分和中间组分主要由负载VLDL的高尔基体液泡和扁平囊组成。几乎排空、常塌陷的高尔基体扁平囊是重组分的主要成分。一种使高尔基体组分在pH 8.5的条件下于法国压榨机中经历低渗休克和剪切的方法,能够提取高尔基体细胞器的内容物,并随后通过差速离心分离其膜。

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