流式细胞术同时检测洋地黄苷渗透细胞线粒体呼吸链活性和活性氧。

N A Pham, B H Robinson, D W Hedley
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引用次数: 96

摘要

背景:呼吸链活性缺陷导致的线粒体活性氧中间体(ROI)生成增加与细胞凋亡等生理过程、线粒体疾病的发病机制以及正常衰老过程有关。已建立的处理呼吸链复合物活性的方法仅限于单个参数的批量测定。本研究描述了一种基于流式细胞术的方法,并验证了该方法对洋地黄苷渗透单细胞呼吸链功能的检测。方法:采用流式细胞术测定不同呼吸条件下线粒体膜电位(DeltaPsi(m))和活性氧生成。这是通过添加底物和抑制剂到洋地黄苷渗透细胞所带来的。通过测量氧气消耗和ATP生成以及共聚焦显微镜验证了该方法。结果:DeltaPsi(m)评估的呼吸链复合物活性对底物和抑制剂的反应与氧气消耗和ATP合成评估的预测一致。此外,流式细胞术方法允许同时评估线粒体ROI生成。这一点通过ROI探针羧基- dcf的定位得到了证实,该定位与共聚焦显微镜观察到的线粒体探针位于同一位置。结论:该方法可以在单细胞水平上研究呼吸链复合物的功能完整性,从而解决呼吸链复合物功能紊乱与线粒体ROI产生之间的关系。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Simultaneous detection of mitochondrial respiratory chain activity and reactive oxygen in digitonin-permeabilized cells using flow cytometry.

Background: Increased mitochondrial generation of reactive oxygen intermediates (ROI) due to defective respiratory chain activity has been implicated in physiological processes such as apoptosis, in the pathogenesis of mitochondrial diseases, and as part of the normal aging process. Established methods addressing activity of the respiratory chain complexes have been limited to bulk assays for single parameters. This study describes a flow cytometry-based method and its validation for the detection of respiratory chain function in single cells permeabilized by digitonin.

Methods: Flow cytometry was used to measure mitochondrial membrane potential (DeltaPsi(m)) and reactive oxygen generation under differing conditions of respiration. This was brought about by the addition of substrates and inhibitors to digitonin-permeabilized cells. This method was validated by measurement of oxygen consumption and ATP production and by confocal microscopy.

Results: Activity of the respiratory chain complexes assessed by DeltaPsi(m) responded to substrates and inhibitors as predicted from assessment by oxygen consumption and ATP synthesis. In addition, the flow cytometry method allows the simultaneous assessment of mitochondrial ROI generation. This was confirmed by the localization of the ROI probe, carboxy-DCF, to the same site as the mitochondrial probe observed by confocal microscopy.

Conclusions: This method allows the functional integrity of the respiratory chain complexes to be studied at the single-cell level, thus addressing the relationship between disordered function of respiratory chain complexes and mitochondrial ROI generation.

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