Darzynkiewicz Z, Bruno S, Del Bino G, Gorczyca W, Hotz M A, Lassota P, Traganos F
Cancer Research Institute, New York Medical College, Valhalla 10595.
Cytometry. 1992;13(8):795-808. doi: 10.1002/cyto.990130802.
The present review describes several methods to characterize and differentiate between two different mechanisms of cell death, apoptosis and necrosis. Most of these methods were applied to studies of apoptosis triggered in the human leukemic HL-60 cell line by DNA topoisomerase I or II inhibitors, and in rat thymocytes by either topoisomerase inhibitors or prednisolone. In most cases, apoptosis was selective to cells in a particular phase of the cell cycle: only S-phase HL-60 cells and G0 thymocytes were mainly affected. Necrosis was induced by excessively high concentrations of these drugs. The following cell features were found useful to characterize the mode of cell death: a) Activation of an endonuclease in apoptocic cells resulted in extraction of the low molecular weight DNA following cell permeabilization, which, in turn, led to their decreased stainability with DNA-specific fluorochromes. Measurements of DNA content made it possible to identify apoptotic cells and to recognize the cell cycle phase specificity of the apoptotic process. b) Plasma membrane integrity, which is lost in necrotic but not apoptotic cells, was probed by the exclusion of propidium iodide (PI). The combination of PI followed by Hoechst 33342 proved to be an excellent probe to distinguish live, necrotic, early- and late-apoptotic cells. c) Mitochondrial transmembrane potential, assayed by retention of rhodamine 123 was preserved in apoptotic but not necrotic cells. d) The ATP-dependent lysosomal proton pump, tested by the supravital uptake of acridine orange (AO) was also preserved in apoptotic but not necrotic cells. e) Bivariate analysis of cells stained for DNA and protein revealed markedly diminished protein content in apoptotic cells, most likely due to activation of endogenous proteases. Necrotic cells, having leaky membranes, had minimal protein content. f) Staining of RNA allowed for the discrimination of G0 from G1 cells and thus made it possible to reveal that apoptosis was selective to G0 thymocytes. g) The decrease in forward light scatter, paralleled either by no change (HL-60 cells) or an increase (thymocytes) of right angle scatter, were early changes during apoptosis. h) The sensitivity of DNA in situ to denaturation, was increased in apoptotic and necrotic cells. This feature, probed by staining with AO at low pH, provided a sensitive and early assay to discriminate between live, apoptotic and necrotic cells, and to evaluate the cell cycle phase specificity of these processes. i) The in situ nick translation assay employing labeled triphosphonucleotides can be used to reveal DNA strand breaks, to detect the very early stages of apoptosis.(ABSTRACT TRUNCATED AT 400 WORDS)
本综述描述了几种表征和区分细胞死亡的两种不同机制——凋亡和坏死的方法。这些方法大多应用于对人白血病HL-60细胞系中由DNA拓扑异构酶I或II抑制剂引发的凋亡研究,以及对大鼠胸腺细胞中由拓扑异构酶抑制剂或泼尼松龙引发的凋亡研究。在大多数情况下,凋亡对细胞周期特定阶段的细胞具有选择性:仅S期HL-60细胞和G0期胸腺细胞主要受到影响。坏死是由这些药物的过高浓度诱导产生的。发现以下细胞特征有助于表征细胞死亡模式:a)凋亡细胞中的核酸内切酶激活导致细胞通透后低分子量DNA的提取,这进而导致它们与DNA特异性荧光染料的染色性降低。DNA含量的测量使得识别凋亡细胞并认识凋亡过程的细胞周期阶段特异性成为可能。b)通过碘化丙啶(PI)排除法检测质膜完整性,质膜完整性在坏死细胞中丧失但在凋亡细胞中未丧失。PI随后用Hoechst 33342染色的组合被证明是区分活细胞、坏死细胞、早期和晚期凋亡细胞的极佳探针。c)通过罗丹明123保留检测的线粒体跨膜电位在凋亡细胞中得以保留但在坏死细胞中未保留。d)通过吖啶橙(AO)的活体摄取测试的ATP依赖性溶酶体质子泵在凋亡细胞中也得以保留但在坏死细胞中未保留。e)对DNA和蛋白质染色的细胞进行双变量分析显示凋亡细胞中的蛋白质含量显著减少,很可能是由于内源性蛋白酶的激活。坏死细胞的膜有渗漏,蛋白质含量最低。f)RNA染色允许区分G0期和G1期细胞,从而有可能揭示凋亡对G0期胸腺细胞具有选择性。g)前向光散射的减少,在HL-60细胞中无变化或在胸腺细胞中增加的直角散射与之平行,是凋亡过程中的早期变化。h)凋亡和坏死细胞中DNA原位对变性的敏感性增加。通过在低pH下用AO染色检测到的这一特征提供了一种灵敏且早期的检测方法,用于区分活细胞、凋亡细胞和坏死细胞,并评估这些过程的细胞周期阶段特异性。i)采用标记三磷酸核苷酸的原位缺口平移测定法可用于揭示DNA链断裂,检测凋亡的极早期阶段。(摘要截短于400字)
