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一种用于制备固定在悬浮液中的细胞以进行扫描电子显微镜检查的高产技术。

A high-yield technique for preparing cells fixed in suspension for scanning electron microscopy.

作者信息

Sanders S K, Alexander E L, Braylan R C

出版信息

J Cell Biol. 1975 Nov;67(2PT.1):476-80. doi: 10.1083/jcb.67.2.476.

Abstract

Human leukocytes fixed in suspension were allowed to settle onto poly-L-lysine-coated glass coverslips and prepared for observation with the scanning electron microscope (SEM). The coverslips were dehydrated in ethanol, critical point dried with CO2, and coated with gold-palladium. With the aid of a locator grid, several fields were photographed with light microscopy after the cells had settled onto the poly-L-lysine-coated coverslips and again after completion of the processing before SEM observation. Quantitative comparison of the number of cells present after settling with the number retained for final viewing with the SEM revealed a cell yield approaching 100%. This simple, reproducible, high-yield technique for processing cells fixed in suspension for SEM prevents changes in surface architecture induced by collecting live cells onto various substrates before fixation and also avoids potentially selective cell losses. Such a technique should allow quantitative correlations between SEM and other morphological and functional parameters.

摘要

将悬浮状态下固定的人白细胞放置在涂有聚-L-赖氨酸的玻璃盖玻片上,然后制备用于扫描电子显微镜(SEM)观察的样本。盖玻片在乙醇中脱水,用二氧化碳进行临界点干燥,再涂上金钯。借助定位网格,在细胞沉降到涂有聚-L-赖氨酸的盖玻片上后,用光学显微镜拍摄了几个视野,在完成SEM观察前的处理后再次拍摄。对沉降后存在的细胞数量与最终用于SEM观察保留的细胞数量进行定量比较,结果显示细胞回收率接近100%。这种用于处理悬浮状态下固定细胞以便进行SEM观察的简单、可重复且高产的技术,可防止在固定前将活细胞收集到各种基质上所引起的表面结构变化,还避免了潜在的选择性细胞损失。这样一种技术应能使SEM与其他形态学和功能参数之间建立定量相关性。

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