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内吞途径的电子显微镜观察

Electron microscopy of endocytic pathways.

作者信息

Ranftler Carmen, Auinger Peter, Meisslitzer-Ruppitsch Claudia, Ellinger Adolf, Neumüller Josef, Pavelka Margit

机构信息

Department of Cell Biology and Ultrastructure Research, Center for Anatomy and Cell Biology, Medical University of Vienna, Vienna, Austria.

出版信息

Methods Mol Biol. 2013;931:437-47. doi: 10.1007/978-1-62703-056-4_22.

Abstract

Detailed insight into the fine structure and 3D-architecture of the complex and dynamic compartments of the endocytic system is essential for a morpho-functional analysis of retrograde traffic from the cell surface to different intracellular destinations. Here, we describe a cytochemical approach for electron microscopic exploration of endocytic pathways with the use of wheat germ agglutinin (WGA) in combination with either conventional chemical fixation or ultrafast physical fixation of the cells by high pressure-freezing. Horseradish peroxidase-labeled WGA endocytozed by human hepatoma cells for various periods of time served as a marker. Its intracellular routes were visualized by means of diaminobenzidine oxidation either done conventionally after chemical fixation or in living cells prior to physical fixation. The latter protocol permits the combination of peroxidase-catalyzed cytochemistry with high pressure-freezing (HPF), which is state of the art for ultrastructural studies of complex and dynamic organelles at high spatial and temporal resolutions. The technique yields distinct cytochemical reactions and excellently preserved fine structures well qualified for detailed electron microscopic and 3D-studies of the complex endocytic architectures.

摘要

深入了解内吞系统复杂且动态的区室的精细结构和三维结构,对于从细胞表面到不同细胞内目的地的逆行运输进行形态功能分析至关重要。在此,我们描述了一种细胞化学方法,用于通过电子显微镜探索内吞途径,该方法使用小麦胚凝集素(WGA),并结合细胞的常规化学固定或通过高压冷冻进行的超快物理固定。人肝癌细胞在不同时间段内内化的辣根过氧化物酶标记的WGA用作标记物。其细胞内途径通过二氨基联苯胺氧化来可视化,这可以在化学固定后常规进行,也可以在物理固定前在活细胞中进行。后一种方案允许将过氧化物酶催化的细胞化学与高压冷冻(HPF)相结合,这是在高空间和时间分辨率下对复杂且动态的细胞器进行超微结构研究的先进技术。该技术产生明显的细胞化学反应,并能出色地保存精细结构,非常适合对复杂的内吞结构进行详细的电子显微镜和三维研究。

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