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使用新型可固定荧光染料分析线粒体形态和功能。

Analysis of mitochondrial morphology and function with novel fixable fluorescent stains.

作者信息

Poot M, Zhang Y Z, Krämer J A, Wells K S, Jones L J, Hanzel D K, Lugade A G, Singer V L, Haugland R P

机构信息

Molecular Probes, Inc., Eugene, Oregon 97402, USA.

出版信息

J Histochem Cytochem. 1996 Dec;44(12):1363-72. doi: 10.1177/44.12.8985128.

DOI:10.1177/44.12.8985128
PMID:8985128
Abstract

Investigation of mitochondrial morphology and function has been hampered because photostable, mitochondrion-specific stains that are retained in fixed, permeabilized cells have not been available. We found that in live cell preparations, the CMXRos and H2-CMXRos dyes were more photostable than rhodamine 123. In addition, fluorescence and morphology of mitochondria stained with the CMXRos and CMXRos-H2 dyes were preserved even after formaldehyde fixation and acetone permeabilization. Using epifluorescence microscopy, we showed that CMXRos and H2-CMXRos dye fluorescence fully co-localized with antibodies to subunit I of cytochrome c oxidase, indicating that the dyes specifically stain mitochondria. Confocal microscopy of these mitochondria yielded colored banding patterns, suggesting that these dyes and the mitochondrial enzyme localize to different suborganellar regions. Therefore, these stains provide powerful tools for detailed analysis of mitochondrial fine structure. We also used poisons that decrease mitochondrial membrane potential and an inhibitor of respiration complex II to show by flow cytometry that the fluorescence intensity of CMXRos and H2-CMXRos dye staining responds to changes in mitochondrial membrane potential and function. Hence, CMXRos has the potential to monitor changes in mitochondrial function. In addition, CMXRos staining was used in conjunction with spectrally distinct fluorescent probes for the cell nucleus and the microtubule network to concomitantly evaluate multiple features of cell morphology.

摘要

线粒体形态和功能的研究一直受到阻碍,因为一直没有可在固定、通透处理的细胞中保留的光稳定、线粒体特异性染料。我们发现,在活细胞制剂中,CMXRos和H2-CMXRos染料比罗丹明123具有更高的光稳定性。此外,即使经过甲醛固定和丙酮通透处理,用CMXRos和CMXRos-H2染料染色的线粒体的荧光和形态仍得以保留。利用落射荧光显微镜,我们发现CMXRos和H2-CMXRos染料荧光与细胞色素c氧化酶亚基I抗体完全共定位,表明这些染料可特异性地对线粒体进行染色。对这些线粒体进行共聚焦显微镜观察产生了彩色条带模式,表明这些染料和线粒体酶定位于不同的亚细胞器区域。因此,这些染料为线粒体精细结构的详细分析提供了强大的工具。我们还使用了降低线粒体膜电位的毒物和呼吸复合体II的抑制剂,通过流式细胞术表明CMXRos和H2-CMXRos染料染色的荧光强度对线粒体膜电位和功能的变化有反应。因此,CMXRos有监测线粒体功能变化的潜力。此外,CMXRos染色与用于细胞核和微管网络的光谱不同的荧光探针结合使用,以同时评估细胞形态的多个特征。

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