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使用 Seahorse XF 分析仪计算 ATP 生成率。

Calculation of ATP production rates using the Seahorse XF Analyzer.

机构信息

Department of Molecular and Medical Pharmacology, University of California, Los Angeles, Los Angeles, CA, USA.

Department of Microbiology, Immunology, and Molecular Genetics, University of California, Los Angeles, Los Angeles, CA, USA.

出版信息

EMBO Rep. 2023 Oct 9;24(10):e56380. doi: 10.15252/embr.202256380. Epub 2023 Aug 7.

Abstract

Oxidative phosphorylation and glycolysis are the dominant ATP-generating pathways in mammalian metabolism. The balance between these two pathways is often shifted to execute cell-specific functions in response to stimuli that promote activation, proliferation, or differentiation. However, measurement of these metabolic switches has remained mostly qualitative, making it difficult to discriminate between healthy, physiological changes in energy transduction or compensatory responses due to metabolic dysfunction. We therefore present a broadly applicable method to calculate ATP production rates from oxidative phosphorylation and glycolysis using Seahorse XF Analyzer data and empirical conversion factors. We quantify the bioenergetic changes observed during macrophage polarization as well as cancer cell adaptation to in vitro culture conditions. Additionally, we detect substantive changes in ATP utilization upon neuronal depolarization and T cell receptor activation that are not evident from steady-state ATP measurements. This method generates a single readout that allows the direct comparison of ATP produced from oxidative phosphorylation and glycolysis in live cells. Additionally, the manuscript provides a framework for tailoring the calculations to specific cell systems or experimental conditions.

摘要

氧化磷酸化和糖酵解是哺乳动物代谢中产生 ATP 的主要途径。这两种途径之间的平衡通常会发生转变,以响应促进激活、增殖或分化的刺激,从而执行细胞特异性功能。然而,这些代谢转换的测量方法大多是定性的,因此很难区分能量转导中健康的、生理性的变化,还是由于代谢功能障碍引起的代偿性反应。因此,我们提出了一种广泛适用的方法,使用 Seahorse XF 分析仪数据和经验转换因子来计算氧化磷酸化和糖酵解产生的 ATP 速率。我们量化了巨噬细胞极化以及癌细胞适应体外培养条件过程中观察到的生物能量变化。此外,我们检测到神经元去极化和 T 细胞受体激活时 ATP 利用的实质性变化,这些变化从稳态 ATP 测量中并不明显。该方法生成一个单一的读数,可以直接比较活细胞中氧化磷酸化和糖酵解产生的 ATP。此外,本文还为针对特定细胞系统或实验条件定制计算提供了一个框架。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ffef/10561364/7608d7c73cd4/EMBR-24-e56380-g006.jpg

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