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通过流式细胞术对完整细胞中线粒体膜电位进行定量测定。

Quantitative assay by flow cytometry of the mitochondrial membrane potential in intact cells.

作者信息

Rottenberg H, Wu S

机构信息

Pathology Department, m.s. 435, Allegheny University of the Health Sciences, MCP/Hahnemann School of Medicine, Broad and Vine streets, Philadelphia, PA 19102, USA.

出版信息

Biochim Biophys Acta. 1998 Sep 16;1404(3):393-404. doi: 10.1016/s0167-4889(98)00088-3.

Abstract

Mitochondrial membrane potential, in situ, is an important indicator of mitochondrial function and dysfunction. Because of recent interest in the role of mitochondria in signaling, cell injury and cell death, there is a need for a convenient, sensitive and accurate method for the measurement of the mitochondrial membrane potential, Deltapsim, in situ, in a heterogeneous cell population. We have adapted a flow cytometry method for the quantitative measurement of DeltaPsim which utilizes the lipophilic, cationic, fluorescent probe 3,3'-dihexyloxacarbocyanine iodide (DiOC6(3)). We developed a new protocol in which cells are equilibrated with very low dye concentrations (<1 nM). Only under these condition, the cell fluorescence appears to be correlated with the magnitude of DeltaPsim, as evident from the sensitivity of the fluorescence to low concentrations of uncouplers, ionophores and inhibitors of the mitochondrial proton pumps. The magnitude of the plasma membrane potential, DeltaPsip, also affects cell fluorescence, and a procedure that corrects for this effect is outlined. This method offers a distinct advantage over existing methods for estimation of Deltapsim by flow cytometry.

摘要

线粒体膜电位,原位,是线粒体功能及功能障碍的一个重要指标。由于近期人们对线粒体在信号传导、细胞损伤和细胞死亡中的作用感兴趣,因此需要一种方便、灵敏且准确的方法来原位测量异质细胞群体中的线粒体膜电位(Δψm)。我们采用了一种流式细胞术方法来定量测量Δψm,该方法利用亲脂性阳离子荧光探针3,3'-二己基氧杂羰花青碘化物(DiOC6(3))。我们开发了一种新方案,其中细胞用极低的染料浓度(<1 nM)进行平衡。只有在这些条件下,细胞荧光似乎才与Δψm的大小相关,这从荧光对低浓度解偶联剂、离子载体和线粒体质子泵抑制剂的敏感性中可以明显看出。质膜电位(Δψp)的大小也会影响细胞荧光,并且概述了一种校正这种影响的程序。该方法相对于现有的通过流式细胞术估计Δψm的方法具有明显优势。

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