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细胞荧光法检测Jurkat T淋巴瘤细胞早期CD95/Fas/APO-1触发凋亡过程中的线粒体变化。七种线粒体特异性荧光染料的比较

Cytofluorometric detection of mitochondrial alterations in early CD95/Fas/APO-1-triggered apoptosis of Jurkat T lymphoma cells. Comparison of seven mitochondrion-specific fluorochromes.

作者信息

Métivier D, Dallaporta B, Zamzami N, Larochette N, Susin S A, Marzo I, Kroemer G

机构信息

Centre National de la Recherche Scientifique, Unité Propre de Recherche 420, Villejuif, France.

出版信息

Immunol Lett. 1998 Apr;61(2-3):157-63. doi: 10.1016/s0165-2478(98)00013-3.

DOI:10.1016/s0165-2478(98)00013-3
PMID:9657269
Abstract

It is commonly accepted that mitochondria undergo major changes early during the apoptotic process and that these alterations are critical for the death/life decision. Here we report that Jurkat T cell leukemia cells exhibit a perturbed incorporation of potential-sensitive fluorochromes. After 6 h of CD95/Fas/APO-1 crosslinking, a significant fraction of still normal-sized Jurkat cells exhibit a decreased incorporation of three different cationic lipophilic dyes commonly used for the quantitation of the mitochondrial transmembrane potential (deltapsi(m)): DiOC6(3), chloromethyl-X-rosamine, and tetramethylrhodaminemethylester. In contrast, upon induction of apoptosis, cells tend to exhibit an increase in the fluorescence obtained with rhodamine 123. The increased rhodamine 123 fluorescence into cells undergoing apoptosis is not affected by labeling in the presence of the protonophore m-chlorophenylhydrazone and thus cannot be attributed to a change in the deltapsi(m). Six hours after CD95 ligation no changes are found among normal-sized cells in the incorporation of mitotracker green and nonylacridine orange, which both measure mitochondrial mass. However, a fraction of cells exhibit an increased staining with the Apo2.7 antibody which detects a mitochondrial antigen generated during apoptosis. These findings underline the importance of using adequate fluorochromes for the quantitation of mitochondrial changes occurring during early apoptosis. Moreover, they cast doubts on those studies that, using rhodamine 123, hypothesized that apoptosis would be associated with a stable or increased deltapsi(m).

摘要

普遍认为线粒体在凋亡过程早期会发生重大变化,且这些改变对于生死抉择至关重要。在此我们报告,Jurkat T细胞白血病细胞对电位敏感荧光染料的掺入存在异常。在CD95/Fas/APO - 1交联6小时后,相当一部分大小仍正常的Jurkat细胞对三种常用于定量线粒体跨膜电位(Δψm)的不同阳离子亲脂性染料的掺入减少:DiOC6(3)、氯甲基 - X - 若丹明和四甲基罗丹明甲酯。相反,在诱导凋亡时,细胞用罗丹明123检测时荧光往往会增加。凋亡细胞中罗丹明123荧光增加不受质子载体间氯苯腙存在时标记的影响,因此不能归因于Δψm的变化。CD95连接6小时后,大小正常的细胞中线粒体质量检测染料Mitotracker green和壬基吖啶橙的掺入未发现变化。然而,一部分细胞用检测凋亡期间产生的线粒体抗原的Apo2.7抗体染色增加。这些发现强调了使用合适的荧光染料定量早期凋亡期间线粒体变化的重要性。此外,它们对那些使用罗丹明123假设凋亡与稳定或增加的Δψm相关的研究提出了质疑。

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