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在冻干细胞骨架的铂复制品中揭示的细丝组织。

Filament organization revealed in platinum replicas of freeze-dried cytoskeletons.

作者信息

Heuser J E, Kirschner M W

出版信息

J Cell Biol. 1980 Jul;86(1):212-34. doi: 10.1083/jcb.86.1.212.

Abstract

This report presents the appearance of rapidly frozen, freeze-dried cytoskeletons that have been rotary replicated with platinum and viewed in the transmission electron microscope. The resolution of this method is sufficient to visualize individual filaments in the cytoskeleton and to discriminate among actin, microtubules, and intermediate filaments solely by their surface substructure. This identification has been confirmed by specific decoration with antibodies and selective extraction of individual filament types, and correlated with light microscope immunocytochemistry and gel electrophoresis patterns. The freeze-drying preserves a remarkable degree of three-dimensionality in the organization of these cytoskeletons. They look strikingly similar to the meshwork of strands or "microtrabeculae" seen in the cytoplasm of whole cells by high voltage electron microscopy, in that the filaments form a lattice of the same configutation and with the same proportions of open area as the microtrabeculae seen in whole cells. The major differences between these two views of the structural elements of the cytoplasmic matrix can be attributed to the effects of aldehyde fixation and dehydration. Freeze-dried cytoskeletons thus provide an opportunity to study--at high resolution and in the absence of problems caused by chemical fixation--the detailed organization of filaments in different regions of the cytoplasm and at different stages of cell development. In this report the pattern of actin and intermediate filament organization in various regions of fully spread mouse fibroblasts is described.

摘要

本报告展示了快速冷冻、冻干的细胞骨架的外观,这些细胞骨架已用铂进行旋转复型,并在透射电子显微镜下观察。该方法的分辨率足以可视化细胞骨架中的单个细丝,并仅通过其表面亚结构区分肌动蛋白、微管和中间丝。通过抗体的特异性标记和对单个细丝类型的选择性提取,已证实了这种识别,并与光学显微镜免疫细胞化学和凝胶电泳图谱相关联。冻干在这些细胞骨架的组织中保留了显著程度的三维结构。它们与通过高压电子显微镜在全细胞细胞质中看到的链状或“微梁”网络惊人地相似,因为细丝形成了与全细胞中看到的微梁相同构型且开放区域比例相同的晶格。细胞质基质结构元件的这两种视图之间的主要差异可归因于醛固定和脱水的影响。因此,冻干的细胞骨架提供了一个机会,以高分辨率且在不存在化学固定引起的问题的情况下,研究细胞质不同区域以及细胞发育不同阶段细丝的详细组织。在本报告中,描述了完全铺展的小鼠成纤维细胞各个区域中肌动蛋白和中间丝组织的模式。

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