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分离出的中心体的结构和化学特征

Structural and chemical characterization of isolated centrosomes.

作者信息

Bornens M, Paintrand M, Berges J, Marty M C, Karsenti E

机构信息

Centre de Génétique Moléculair, CNRS, Gif-sur-Yvette, France.

出版信息

Cell Motil Cytoskeleton. 1987;8(3):238-49. doi: 10.1002/cm.970080305.

Abstract

A procedure adapted from that described by Mitchison and Kirschner [Nature 312:232-237, 1984] was used to isolate centrosomes from human lymphoid cells. High yields of homogeneous centrosomes (60% of the theoretical total, assuming one centrosome per cell) were obtained. Centrosomes were isolated as pairs of centrioles, plus their associated pericentriolar material. Ultrastructural investigation revealed: 1) a link between both centrioles in a centrosome formed by the gathering in of a unique bundle of thin filaments surrounding each centriole; 2) a stereotypic organization of the pericentriolar material, including a rim of constant width at the proximal end of each centriole and a disc of nine satellite arms organized according to a ninefold symmetry at the distal end and; 3) an axial hub in the lumen of each centriole at the distal end surrounded by some ill-defined material. The total protein content was 2 to 3 X 10(-2) pg per isolated centrosome, a figure that suggests that the preparations were close to homogeneity. The protein composition was complex but specific, showing proteins ranging from 180 to 300 kD, one prominent band at 130 kD, and a group of proteins between 50 and 65 kD. Actin was also present in centrosome preparations. Functional studies demonstrated that the isolated centrosomes were competent to nucleate microtubules in vitro from purified tubulin in conditions in which spontaneous assembly could not occur. They were also very effective at inducing cleavage when microinjected into unfertilized Xenopus eggs.

摘要

采用了一种改编自米奇森和基尔施纳所描述方法(《自然》312:232 - 237, 1984)的程序,从人淋巴细胞中分离中心体。获得了高产率的均一中心体(假设每个细胞有一个中心体,产量为理论总量的60%)。中心体作为一对中心粒及其相关的中心粒周围物质被分离出来。超微结构研究显示:1)在一个中心体中的两个中心粒之间存在一种联系,这种联系由围绕每个中心粒聚集的一束独特的细丝形成;2)中心粒周围物质具有刻板的组织形式,包括每个中心粒近端有一个宽度恒定的边缘,以及在远端有一个按九重对称组织的由九个卫星臂组成的盘状物;3)在每个中心粒远端的管腔内有一个轴向中心体,周围是一些不明确的物质。每个分离的中心体的总蛋白含量为2至3×10⁻²皮克,这一数字表明制备物接近均一性。蛋白质组成复杂但具有特异性,显示出分子量范围从180至300千道尔顿的蛋白质,一条在130千道尔顿处的突出条带,以及一组分子量在50至65千道尔顿之间的蛋白质。肌动蛋白也存在于中心体制备物中。功能研究表明,分离的中心体在体外能够在无法发生自发组装的条件下,从纯化的微管蛋白中使微管成核。当将它们显微注射到未受精的非洲爪蟾卵中时,它们在诱导卵裂方面也非常有效。

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