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在流式细胞仪测量电子细胞体积过程中DNA荧光染料的电解降解

Electrolytic degradation of DNA fluorochromes during flow cytometric measurement of electronic cell volume.

作者信息

Alabaster O, Glaubiger D L, Hamilton V T, Bentley S A, Shackney S E, Skramstad K S, Chen R F

出版信息

J Histochem Cytochem. 1980 Apr;28(4):330-4. doi: 10.1177/28.4.6445379.

Abstract

Changes in flow cytometric measurement of DNA content can result from electrolytic chemical degradation of mithramycin, ethidium bromide, and propidium iodide during simultaneous measurement of electronic cell volume. Bench electrolysis also degrades these fluorochromes without changing the quantum yields, even when they are complexed to DNA. In the flow cytometer, electrolytic production of chlorine at the anode is the probable cause of this degradation, since exposure of these fluorochromes to chlorine gas produces the same effect. It is therefore advisable to measure the DNA content distribution alone before simultaneously measuring the DNA content and the electronic cell volume. If unavoidable effects on the DNA distribution are present, narrow forward-angle light scatter should be used as the cell size indicator during dual parameter measurements. Modifying instrument design by reversing electrode polarity might eliminate this problem.

摘要

在同时测量电子细胞体积过程中,放线菌素、溴化乙锭和碘化丙啶的电解化学降解会导致DNA含量的流式细胞术测量结果发生变化。台式电解也会降解这些荧光染料,即使它们与DNA结合,也不会改变量子产率。在流式细胞仪中,阳极处电解产生氯气可能是这种降解的原因,因为这些荧光染料暴露于氯气会产生相同的效果。因此,建议在同时测量DNA含量和电子细胞体积之前,单独测量DNA含量分布。如果对DNA分布存在不可避免的影响,在双参数测量期间应使用窄前向角光散射作为细胞大小指标。通过反转电极极性来修改仪器设计可能会消除这个问题。

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