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Membrane skeleton in fresh unfixed erythrocytes as revealed by a rapid-freezing and deep-etching method.

机译:通过快速冷冻和深蚀刻方法揭示的新鲜未固定红细胞的膜骨架。

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摘要

A rapid-freezing and deep-etching method for examining en face the cytoplasmic aspects of unfixed erythrocyte membranes is described, which provides improved resolution. Normal human erythrocytes were centrifuged, washed in a phosphate buffer solution and pelleted. Glass coverslips were coated with 3-aminopropyl triethoxy silane and glutaraldehyde to make erythrocytes stick to them. A drop containing the erythrocyte pellet was sandwiched between 2 coverslips. The attached erythrocytes were slowly split open in the cytosol buffer solution. The specimens on coverslips were rapidly frozen in an isopentane-propane mixture (-193 degrees C), deeply etched and rotary shadowed with platinum and carbon. Filamentous structures were observed to form fine networks on the cytoplasmic side of erythrocyte membranes. The length of the filaments was shorter than that previously reported for glutaraldehyde-fixed filaments. The number of intersections between filaments was increased as compared with the previous data. It is concluded that dense in situ networks of short filaments beneath erythrocyte membranes can be viewed in a relatively intact state by splitting fresh unfixed specimens followed by the rapid-freezing and deep-etching method.
机译:描述了用于检查未固定的红细胞膜的细胞质方面的快速冷冻和深蚀刻方法,其提供了改善的分辨率。将正常人的红细胞离心,在磷酸盐缓冲液中洗涤并沉淀。在玻璃盖玻片上涂上3-氨丙基三乙氧基硅烷和戊二醛,使红细胞粘附在其上。将含有红细胞沉淀的液滴夹在两个盖玻片之间。将附着的红细胞在细胞溶质缓冲液中缓慢分裂开。将盖玻片上的样品在异戊烷-丙烷混合物(-193摄氏度)中快速冷冻,进行深度蚀刻并用铂和碳旋转遮盖。观察到丝状结构在红细胞膜的细胞质侧形成精细的网络。细丝的长度比以前报道的戊二醛固定细丝的长度短。与以前的数据相比,细丝之间的相交数量增加了。结论是,通过分裂新鲜的未固定标本,然后进行快速冷冻和深蚀刻方法,可以在相对完整的状态下观察红细胞膜下方短丝的密集原位网络。

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