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体外功能性中心体的拆卸与重新组装。

The disassembly and reassembly of functional centrosomes in vitro.

作者信息

Schnackenberg B J, Khodjakov A, Rieder C L, Palazzo R E

机构信息

Department of Biochemistry, Cell, and Molecular Biology, University of Kansas, Lawrence, KS 66045, USA.

出版信息

Proc Natl Acad Sci U S A. 1998 Aug 4;95(16):9295-300. doi: 10.1073/pnas.95.16.9295.

Abstract

Animal cells contain a single centrosome that nucleates and organizes a polarized array of microtubules which functions in many cellular processes. In most cells the centrosome is composed of two centrioles surrounded by an ill-defined "cloud" of pericentriolar material. Recently, gamma-tubulin-containing 25-nm diameter ring structures have been identified as likely microtubule nucleation sites within the pericentriolar material of isolated centrosomes. Here we demonstrate that when Spisula centrosomes are extracted with 1.0 M KI they lose their microtubule nucleation potential and appear by three-dimensional electron microscopy as a complex lattice, built from 12- to 15-nm thick elementary fiber(s), that lack centrioles and 25-nm rings. Importantly, when these remnants are incubated in extracts prepared from Spisula oocytes they recover their 25-nm rings, gamma-tubulin, and microtubule nucleation potential. This recovery process occurs in the absence of microtubules, divalent cations, and nucleotides. Thus, in animals the centrosome is structurally organized around a KI-insoluble filament-based "centromatrix" that serves as a scaffold to which those proteins required for microtubule nucleation bind, either directly or indirectly, in a divalent cation and nucleotide independent manner.

摘要

动物细胞含有单个中心体,该中心体可形成并组织极化的微管阵列,其在许多细胞过程中发挥作用。在大多数细胞中,中心体由两个中心粒组成,周围环绕着界限不明确的中心粒周围物质“云”。最近,已确定直径为25纳米、含γ-微管蛋白的环状结构可能是分离出的中心体的中心粒周围物质内的微管成核位点。在此,我们证明,用1.0 M KI提取缢蛏中心体时,它们会失去微管成核潜力,并且通过三维电子显微镜观察,其呈现为由12至15纳米厚的基本纤维构成的复杂晶格,其中没有中心粒和25纳米的环。重要的是,当将这些残余物在缢蛏卵母细胞制备的提取物中孵育时,它们会恢复其25纳米的环、γ-微管蛋白和微管成核潜力。这种恢复过程在没有微管、二价阳离子和核苷酸的情况下发生。因此,在动物中,中心体在结构上围绕基于KI不溶性细丝的“中心基质”组织,该“中心基质”作为支架,微管成核所需的那些蛋白质以二价阳离子和核苷酸独立的方式直接或间接结合到该支架上。

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