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沿微管带的囊泡运输以及从草履虫中分离胞质动力蛋白。

Vesicle transport along microtubular ribbons and isolation of cytoplasmic dynein from Paramecium.

作者信息

Schroeder C C, Fok A K, Allen R D

机构信息

Pacific Biomedical Research Center, University of Hawaii, Honolulu 96822.

出版信息

J Cell Biol. 1990 Dec;111(6 Pt 1):2553-62. doi: 10.1083/jcb.111.6.2553.

Abstract

Cytoplasmic microtubule-based motility in Paramecium was investigated using video-enhanced contrast microscopy, the quick-freeze, deep-etch technique, and biochemical isolations. Three distinct vesicle populations were found to be transported unidirectionally along the cytopharyngeal microtubular ribbons. This minus-end-directed movement exhibited unique in vivo features in that the vesicle transport was nonsaltatory, rapid, and predominantly along one side of the microtubular ribbons. To identify candidate motor proteins which may participate in vesicle transport, we prepared cytosolic extracts of Paramecium and used bovine brain microtubules as an affinity matrix. These preparations were found to contain a microtubule-stimulated ATPase which supported microtubule gliding in vitro. This protein was verified as a cytoplasmic dynein based upon its relative molecular mass, sedimentation coefficient of 16S, susceptibility to vanadate photocleavage, elevated CTPase/ATPase ratio, and its typical two-headed dynein morphology. This dynein was directly compared with the axonemal dyneins from Paramecium and found to differ by five criteria: morphology, sedimentation coefficient, CTPase/ATPase ratio, vanadate cleavage patterns, and polypeptide composition. The cytoplasmic dynein is therefore not an axonemal dynein precursor, but rather it represents a candidate for supporting the microtubule-based vesicle transport which proceeds along the microtubular ribbons.

摘要

利用视频增强对比显微镜、快速冷冻-深度蚀刻技术和生化分离方法,对草履虫中基于细胞质微管的运动进行了研究。发现有三种不同的囊泡群体沿胞咽微管带单向运输。这种向负端的运动在体内表现出独特的特征,即囊泡运输是非跳跃性的、快速的,并且主要沿着微管带的一侧进行。为了鉴定可能参与囊泡运输的候选运动蛋白,我们制备了草履虫的胞质提取物,并使用牛脑微管作为亲和基质。发现这些制剂含有一种微管刺激的ATP酶,它在体外支持微管滑动。根据其相对分子质量、16S的沉降系数、对钒酸盐光裂解的敏感性、升高的CTP酶/ATP酶比率以及其典型的双头动力蛋白形态,该蛋白被确认为细胞质动力蛋白。将这种动力蛋白与草履虫的轴丝动力蛋白直接比较,发现它们在五个标准上存在差异:形态、沉降系数、CTP酶/ATP酶比率、钒酸盐裂解模式和多肽组成。因此,细胞质动力蛋白不是轴丝动力蛋白的前体,而是支持沿微管带进行的基于微管的囊泡运输的候选蛋白。

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