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单层细胞培养物流式细胞荧光术的快速低渗方法。染色和数据分析中的一些陷阱。

Rapid hypotonic method for flow cytofluorometry of monolayer cell cultures. Some pitfalls in staining and data analysis.

作者信息

Fried J, Perez A G, Clarkson B D

出版信息

J Histochem Cytochem. 1978 Nov;26(11):921-33. doi: 10.1177/26.11.82573.

Abstract

The rapid hypotonic staining procedure developed by Krishan for DNA determinations by flow cytofluorometry has been proven accurate for in vivo cell samples and for cell lines growing in suspension culture. We show that the unmodified procedure may produce distorted DNA histograms when used for staining cells growing in monolayer cultures, however. To eliminate these distortions, it was necessary to avoid the use of trypsin by staining the attached cells directly, using a hypotonic fluorochrome solution to which nonionic detergent was added. Two sublines of HeLa S3 cells are shown to exhibit major differences in their staining characteristics. By using our revised staining procedure, the two sublines appear to produce very satisfactory DNA histograms. However, in only one subline does the S phase fraction calculated from the histograms agree with the autoradiographical labeling index. Mitotic cells remain intact under these staining conditions, and the principal observed effect of nonionic detergents in this case is to decrease the coefficient of variation of fluorescence intensity.

摘要

克里山开发的用于通过流式细胞荧光术进行DNA测定的快速低渗染色程序,已被证明对体内细胞样本和悬浮培养中生长的细胞系是准确的。然而,我们发现,当将未修改的程序用于单层培养中生长的细胞染色时,可能会产生扭曲的DNA直方图。为了消除这些扭曲,有必要通过直接对贴壁细胞进行染色来避免使用胰蛋白酶,使用添加了非离子洗涤剂的低渗荧光染料溶液。结果表明,HeLa S3细胞的两个亚系在染色特性上表现出主要差异。通过使用我们修订的染色程序,这两个亚系似乎产生了非常令人满意的DNA直方图。然而,从直方图计算出的S期分数仅在一个亚系中与放射自显影标记指数一致。在这些染色条件下,有丝分裂细胞保持完整,在这种情况下,非离子洗涤剂观察到的主要作用是降低荧光强度的变异系数。

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