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测量人皮肤成纤维细胞中的氧化磷酸化。

Measuring oxidative phosphorylation in human skin fibroblasts.

机构信息

Center for Mitochondrial Disease, Department of Pharmacology, Case Western Reserve University School of Medicine, Cleveland, OH 44106, USA.

出版信息

Anal Biochem. 2013 Jun 1;437(1):52-8. doi: 10.1016/j.ab.2013.02.010. Epub 2013 Feb 24.

Abstract

An approach has been developed to quantitate oxidative phosphorylation in harvested human skin fibroblasts that have been permeabilized with digitonin. In protocol 1, state 3 rates are measured with complex I and II substrates, followed by uncoupled maximal oxidative capacity measured in the presence of these combined substrates as well as through complex IV. In protocol 2, state 3 rates are measured using palmitoylcarnitine to monitor fatty acid oxidation and duroquinol to assess the flux through complex III; uncoupled duroquinol oxidation measures maximal oxidative capacity through complex III. The activity of citrate synthase is determined in every experiment as a marker of the amount of mitochondria per chamber. Data are expressed on the basis of cell count (per million fibroblasts), of protein, or of citrate synthase activity. Cell growth conditions are optimized, and it is necessary to keep cultured cells from reaching confluency. Cultures in passages 3 to 10 show reproducible oxidative phosphorylation data. Based on the data from the 15 normal human skin fibroblast lines, we are evaluating the use of this approach to diagnose systemic mitochondrial disease and avoid issues associated with open skeletal muscle biopsy.

摘要

已开发出一种方法来定量分析已用刀豆球蛋白 A 通透化的人皮肤成纤维细胞中的氧化磷酸化。在方案 1 中,使用复合物 I 和 II 的底物测量状态 3 速率,然后在这些组合底物以及复合物 IV 的存在下测量未偶联的最大氧化能力。在方案 2 中,使用棕榈酰肉碱测量状态 3 速率以监测脂肪酸氧化,并使用二氢奎尼醇评估通过复合物 III 的通量;未偶联的二氢奎尼醇氧化通过复合物 III 测量最大氧化能力。在每个实验中都测定柠檬酸合酶的活性作为每个室中线粒体数量的标志物。数据以细胞计数(每百万成纤维细胞)、蛋白质或柠檬酸合酶活性为基础表示。优化细胞生长条件,必须防止培养细胞达到汇合。第 3 至 10 代的培养物显示出可重复的氧化磷酸化数据。基于来自 15 个人类皮肤成纤维细胞系的数据,我们正在评估使用这种方法来诊断系统性线粒体疾病并避免与开放骨骼肌活检相关的问题。

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