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扫描电子显微镜(SEM)培养细胞的固定、脱水、干燥及镀膜

The fixation, dehydration, drying and coating of cultured cells of SEM.

作者信息

Brunk U, Collins V P, Arro E

出版信息

J Microsc. 1981 Aug;123(Pt 2):121-31. doi: 10.1111/j.1365-2818.1981.tb01288.x.

DOI:10.1111/j.1365-2818.1981.tb01288.x
PMID:6799651
Abstract

Cultivated cells form a valuable model system for studies on the effects of various preparative protocols for scanning electron microscopy (SEM). The various effects of each preparative step can be followed in detail in the light microscope and no diffusion gradients complicate the fixation and other procedures as in the case of solid tissues. Studies on cultivated cells indicate that the glutaraldehyde component of a glutaraldehyde-based fixative does not contribute to the effective osmotic pressure of the fixative and thus the osmolarity of the buffer, and other components, must be equalized to that of the medium in which the cells grow. Even small deviations from this ideal effective osmotic pressure will result in osmotically induced artefacts. Disturbances of pH and temperature of the cultures prior to and during fixation will result in changes in the appearance of many cellular structures such as microspikes and ruffles. We find that osmium fixation is advisable in most instances for best possible membrance preservation and that even long periods of glutaraldehyde fixation do not compensate for osmium fixation. Dehydration always results in shrinkage. Freeze drying (FD) and critical point drying (CPD) also give rise to shrinkage, the former to a lesser degree than the latter. A gold-palladium alloy gives a less granular coating that does gold alone. When cultured cells are studied, a metal thickness of between 5 and 15 nm is usually sufficient to give rise to an adequate secondary electron production and to avoid charging even at accelerating voltages of 30-40 kV. Without treatment with OsO4 a thicker metal coating is required.

摘要

培养细胞为研究扫描电子显微镜(SEM)各种制备方案的效果提供了一个有价值的模型系统。每个制备步骤的各种效果可以在光学显微镜下详细追踪,并且不会像在实体组织中那样,扩散梯度使固定和其他程序复杂化。对培养细胞的研究表明,基于戊二醛的固定剂中的戊二醛成分对固定剂的有效渗透压没有贡献,因此缓冲液和其他成分的渗透压必须与细胞生长的培养基的渗透压相等。即使与这个理想的有效渗透压有很小的偏差也会导致渗透压诱导的假象。固定前和固定过程中培养物的pH值和温度的干扰会导致许多细胞结构如微刺和褶皱的外观发生变化。我们发现,在大多数情况下,锇固定对于尽可能好地保存膜是可取的,而且即使长时间的戊二醛固定也不能弥补锇固定。脱水总是会导致收缩。冷冻干燥(FD)和临界点干燥(CPD)也会导致收缩,前者的程度比后者小。金钯合金涂层比单独的金涂层颗粒更少。当研究培养细胞时,5到15纳米之间的金属厚度通常足以产生足够的二次电子,并即使在30 - 40千伏的加速电压下也能避免充电。未经OsO4处理时,需要更厚的金属涂层。

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