首页> 外文期刊>Progress in Neuro-Psychopharmacology & Biological Psychiatry: An International Research, Review and News Journal >A simple, informative, and quantitative flow cytometric method for assessing apoptosis in cultured cells.
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A simple, informative, and quantitative flow cytometric method for assessing apoptosis in cultured cells.

机译:一种用于评估培养细胞凋亡的简单,信息量和定量流式细胞仪方法。

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摘要

Described herein is a method for assessing apoptosis in tissue culture cells that is facile, highly informative, readily quantifiable, and generally applicable. As in conventional DNA-based flow cytometric analysis, the approach utilizes fixed, propidium iodide-stained cells. However, this particular application employs correlated two-parameter analyses of log(10)DNA fluorescence signals versus log(10) side-scatter (SS) signals of cells undergoing apoptosis. The features and the advantages of this approach, which provides substantially more information than is otherwise available from conventional analysis, are demonstrated in experiments monitoring the effects of the antineoplastic agents cisplatinum (cisP) and camptothecin (CAM) on a variety of cultured cell types, including epithelial cells (SW480; human colon carcinoma), fibroblasts (rat2 and 3T3; normal fibroblast lines), and cells of myeloid origin (CCRF-CEM; human leukemia). The utility of the technique is demonstrated further in a series of experiments with the histidine analogue L-histidinol. These experiments reveal that L-histidinol is pro-apoptotic in CCRF-CEM cells, accentuates markedly the apoptotic response otherwise elicited by CAM in murine B16f10 melanoma cells and inhibits CAM-induced apoptosis in normal 3T3 fibroblasts.
机译:本文描述了一种用于评估组织培养细胞中的细胞凋亡的方法,该方法是容易的,高度有用的,易于量化的并且是普遍适用的。与传统的基于DNA的流式细胞术分析一样,该方法利用固定的碘化丙啶染色细胞。但是,此特定应用程序采用了对log(10)DNA荧光信号与经历凋亡的细胞的log(10)侧向散射(SS)信号进行相关的两参数分析。与常规分析相比,此方法可提供更多的信息,其方法和优点在监视抗肿瘤药顺铂(cisP)和喜树碱(CAM)对多种培养细胞类型的影响的实验中得到了证明,包括上皮细胞(SW480;人结肠癌),成纤维细胞(rat2和3T3;正常成纤维细胞系)和骨髓来源的细胞(CCRF-CEM;人白血病)。使用组氨酸类似物L-组蛋白醇的一系列实验进一步证明了该技术的实用性。这些实验表明,L-组蛋白醇在CCRF-CEM细胞中具有促凋亡作用,可显着增强CAM诱导的鼠B16f10黑色素瘤细胞的凋亡反应,并抑制CAM诱导的正常3T3成纤维细胞凋亡。

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