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培养肝细胞细胞骨架的三维研究:快速冷冻和深度蚀刻研究。

Three-dimensional studies of the cytoskeleton of cultured hepatocytes: a quick-freezing and deep-etching study.

作者信息

Ohno S, Fujii Y

机构信息

Department of Anatomy, Shinshu University School of Medicine, Matsumoto, Japan.

出版信息

Virchows Arch A Pathol Anat Histopathol. 1991;418(1):61-70. doi: 10.1007/BF01600245.

Abstract

The ultrastructure of the cytoskeleton of cultured mouse hepatocytes was studied by a quick-freezing and deep-etching method. Isolated mouse hepatocytes were cultured on collagen gels for 48 h, fixed in paraformaldehyde and centrifuged to prepare cell pellets. The hepatocytes were split open to remove cytoplasmic soluble proteins for replica preparations. Some specimens were decorated with anti-actin antibody or S1 myosin fragments to identify actin filaments. They were quickly frozen in isopentane-propane mixture, fractured in liquid nitrogen, deeply etched in a freeze-fracture machine and rotary shadowed by platinum and carbon. The basal cell membranes of hepatocytes were in contact with the collagen gels and the apical surface faced the culture medium. Networks of actin filaments were attached to the apical cell membranes, but intermediate filaments were localized along the basal layer. Some intermediate filaments were associated with cell organelles, such as the endoplasmic reticulum. The Golgi apparatus was less associated with the cytoskeleton and showed synthesized materials in the cisternae. Cytoskeletal organization in cultured hepatocytes was revealed three-dimensionally, indicating that the interaction of cell membranes with collagen gels is important for the organization of the cytoskeleton.

摘要

采用快速冷冻和深度蚀刻法研究了培养的小鼠肝细胞细胞骨架的超微结构。将分离的小鼠肝细胞在胶原凝胶上培养48小时,用多聚甲醛固定并离心制备细胞沉淀。将肝细胞裂解以去除细胞质可溶性蛋白用于复制品制备。一些标本用抗肌动蛋白抗体或S1肌球蛋白片段进行标记以识别肌动蛋白丝。它们在异戊烷 - 丙烷混合物中快速冷冻,在液氮中断裂,在冷冻断裂机中深度蚀刻,并用铂和碳进行旋转阴影处理。肝细胞的基底细胞膜与胶原凝胶接触,顶端表面面向培养基。肌动蛋白丝网络附着在顶端细胞膜上,但中间丝位于基底层。一些中间丝与细胞器如内质网相关。高尔基体与细胞骨架的关联较少,在潴泡中显示有合成物质。三维揭示了培养肝细胞中的细胞骨架组织,表明细胞膜与胶原凝胶的相互作用对细胞骨架的组织很重要。

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