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在海马实验中测量分离的过氧化物酶体氧化能力的方法。

Methodology for measuring oxidative capacity of isolated peroxisomes in the Seahorse assay.

作者信息

Stork Brittany A, Dean Adam, York Brian

机构信息

Molecular and Cellular Biology, Baylor College of Medicine, Houston, TX 77030, USA.

Dan L. Duncan Cancer Center, Baylor College of Medicine, Houston, TX 77030, USA.

出版信息

J Biol Methods. 2022 Jun 8;9(2):e160. doi: 10.14440/jbm.2022.374. eCollection 2022.

Abstract

The regulation of cellular energetics is a complex process that requires the coordinated function of multiple organelles. Historically, studies focused on understanding cellular energy utilization and production have been overwhelmingly concentrated on the mitochondria. While mitochondria account for the majority of intracellular energy production, they alone are incapable of maintaining the variable energetic demands of the cell. The peroxisome has recently emerged as a secondary metabolic organelle that complements and improves mitochondrial performance. Although mitochondria and peroxisomes are structurally distinct organelles, they share key functional similarities that allows for the potential to repurpose readily available tools initially developed for mitochondrial assessment to interrogate peroxisomal metabolic function in a novel manner. To this end, we report here on procedures for the isolation, purification and real-time metabolic assessment of peroxisomal β-oxidation using the Agilent Seahorse system. When used together, these protocols provide a straightforward, reproducible and highly quantifiable method for measuring the contributions of peroxisomes to cellular and organismal metabolism.

摘要

细胞能量学的调节是一个复杂的过程,需要多个细胞器的协同作用。从历史上看,专注于理解细胞能量利用和产生的研究绝大多数都集中在线粒体上。虽然线粒体占细胞内能量产生的大部分,但仅靠它们自身无法满足细胞不断变化的能量需求。过氧化物酶体最近已成为一种辅助代谢细胞器,可补充并改善线粒体的功能。尽管线粒体和过氧化物酶体在结构上是不同的细胞器,但它们具有关键的功能相似性,这使得最初为线粒体评估而开发的现有工具有可能被重新用于以一种新的方式探究过氧化物酶体的代谢功能。为此,我们在此报告使用安捷伦海马系统进行过氧化物酶体β-氧化的分离、纯化和实时代谢评估的程序。这些方案一起使用时,为测量过氧化物酶体对细胞和机体代谢的贡献提供了一种直接、可重复且高度可量化的方法。

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