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使用改良的BrdU- Hoechst方法对染色体和细胞进行流式细胞术分析。

Flow cytometric analysis of chromosomes and cells using a modified BrdU-Hoechst method.

作者信息

Severin E, Ohnemus B

出版信息

Histochemistry. 1982;76(1):113-21. doi: 10.1007/BF00493290.

Abstract

Chromosomes and interphase cells were harvested from cultures of the Chinese hamster line B14 F28 grown in medium containing BrdU up to four cell cycles and stained with the fluorescent dye 33342 Hoechst for flow cytometry. The newly synthetized BrdU-DNA is not stainable by the Hoechst dye which is highly specific for thymidine. The temporal development of the DNA fluorescence after addition of BrdU to the growth medium has been investigated. The chromosomal fluorescence intensity is reduced one step per generation. The extent of the intensity decrease by BrdU incorporation is proportional to the amount of new DNA and it is realized by repeated measurement following an UV-exposure. This UV-illumination stops the quenching by BrdU of the Hoechst stain induced DNA fluorescence. Therefore, the entire DNA content of these chromosomes now becomes measurable. The obtained intensity gain serves as a measure of the extent of the previous BrdU caused intensity shift. In this way we could establish 3 successive mitoses. Principally, this method is suitable also for measurement of whole cells in order to obtain both the number of generations in the experimental period and the phase distribution of the cell cycle.

摘要

从在含有BrdU的培养基中培养至四个细胞周期的中国仓鼠B14 F28细胞系培养物中收获染色体和间期细胞,并用荧光染料Hoechst 33342进行染色,用于流式细胞术分析。新合成的BrdU-DNA不能被对胸腺嘧啶具有高度特异性的Hoechst染料染色。研究了在生长培养基中添加BrdU后DNA荧光的时间变化。染色体荧光强度每代降低一级。通过BrdU掺入导致的强度降低程度与新DNA的量成正比,并且通过紫外线照射后的重复测量来实现。这种紫外线照射停止了BrdU对Hoechst染色诱导的DNA荧光的淬灭作用。因此,这些染色体的全部DNA含量现在变得可测量。获得的强度增加用作先前BrdU引起的强度变化程度的度量。通过这种方式,我们可以确定3个连续的有丝分裂。原则上,该方法也适用于全细胞的测量,以便获得实验期间的代数和细胞周期的阶段分布。

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