首页> 美国卫生研究院文献>Journal of Visualized Experiments : JoVE >Plunge Freezing: A Tool for the Ultrastructural and Immunolocalization Studies of Suspension Cells in Transmission Electron Microscopy
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Plunge Freezing: A Tool for the Ultrastructural and Immunolocalization Studies of Suspension Cells in Transmission Electron Microscopy

机译:急冻:透射电子显微镜中悬浮细胞的超微结构和免疫定位研究的工具

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摘要

Transmission Electron Microscopy (TEM) is an extraordinary tool for studying cell ultrastructure, in order to localize proteins and visualize macromolecular complexes at very high resolution. However, to get as close as possible to the native state, perfect sample preservation is required. Conventional electron microscopy (EM) fixation with aldehydes, for instance, does not provide good ultrastructural preservation. The slow penetration of fixatives induces cell reorganization and loss of various cell components. Therefore, conventional EM fixation does not allow for an instantaneous stabilization and preservation of structures and antigenicity. The best choice for examining intracellular events is to use cryofixation followed by the freeze-substitution fixation method that keeps cells in their native state. High-pressure freezing/freeze-substitution, which preserves the integrity of cellular ultrastructure, is the most commonly used method, but requires expensive equipment. Here, an easy-to-use and low-cost freeze fixation method followed by freeze-substitution for suspension cell cultures is presented.
机译:透射电子显微镜(TEM)是研究细胞超微结构的非凡工具,可以以非常高的分辨率定位蛋白质并可视化大分子复合物。但是,为了尽可能接近原始状态,需要完美的样品保存。例如,常规的用醛固定的电子显微镜(EM)不能提供良好的超微结构保存。固定剂的缓慢渗透诱导细胞重组和各种细胞成分的损失。因此,常规的EM固定不允许瞬时稳定和保存结构和抗原性。检查细胞内事件的最佳选择是使用冷冻固定,然后使用冷冻替代固定方法,使细胞保持其原始状态。保留细胞超微结构完整性的高压冷冻/冷冻替代是最常用的方法,但需要昂贵的设备。在这里,提出了一种易于使用且成本低廉的冷冻固定方法,然后采用冷冻替代法进行悬浮细胞培养。

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