洋地黄素
线粒体
生物化学
细胞外
谷氨酰胺
生物
呼吸链
生物能学
选择性氧化酶
线粒体呼吸链
细胞生物学
焊剂(冶金)
生物物理学
化学
膜
氨基酸
有机化学
作者
Joshua K. Salabei,Andrew Gibb,Bradford G. Hill
出处
期刊:Nature Protocols
[Nature Portfolio]
日期:2014-01-23
卷期号:9 (2): 421-438
被引量:323
标识
DOI:10.1038/nprot.2014.018
摘要
Extracellular flux (XF) analysis has become a mainstream method for measuring mitochondrial function in cells and tissues. Although this technique is commonly used to measure bioenergetics in intact cells, we outline here a detailed XF protocol for measuring respiration in permeabilized cells. Cells are permeabilized using saponin (SAP), digitonin (DIG) or recombinant perfringolysin O (rPFO) (XF-plasma membrane permeabilizer (PMP) reagent), and they are provided with specific substrates to measure complex I– or complex II–mediated respiratory activity, complex III+IV respiratory activity or complex IV activity. Medium- and long-chain acylcarnitines or glutamine may also be provided for measuring fatty acid (FA) oxidation or glutamine oxidation, respectively. This protocol uses a minimal number of cells compared with other protocols and does not require isolation of mitochondria. The results are highly reproducible, and mitochondria remain well coupled. Collectively, this protocol provides comprehensive and detailed information regarding mitochondrial activity and efficiency, and, after preparative steps, it takes 6–8 h to complete.
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