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新鲜分离的小鼠肝细胞悬浮液中脂肪酸 β-氧化的测定。

Measurement of Fatty Acid β-Oxidation in a Suspension of Freshly Isolated Mouse Hepatocytes.

机构信息

Department of Biochemistry, School of Medicine, West Virginia University.

Department of Biochemistry, School of Medicine, West Virginia University;

出版信息

J Vis Exp. 2021 Sep 9(175). doi: 10.3791/62904.

Abstract

Fatty acid β-oxidation is a key metabolic pathway to meet the energy demands of the liver and provide substrates and cofactors for additional processes, such as ketogenesis and gluconeogenesis, which are essential to maintain whole-body glucose homeostasis and support extra-hepatic organ function in the fasted state. Fatty acid β-oxidation occurs within the mitochondria and peroxisomes and is regulated through multiple mechanisms, including the uptake and activation of fatty acids, enzyme expression levels, and availability of cofactors such as coenzyme A and NAD. In assays that measure fatty acid β-oxidation in liver homogenates, cell lysis and the common addition of supraphysiological levels of cofactors mask the effects of these regulatory mechanisms. Furthermore, the integrity of the organelles in the homogenates is hard to control and can vary significantly between preparations. The measurement of fatty acid β-oxidation in intact primary hepatocytes overcomes the above pitfalls. This protocol describes a method for the measurement of fatty acid β-oxidation in a suspension of freshly isolated primary mouse hepatocytes incubated with C-labeled palmitic acid. By avoiding hours to days of culture, this method has the advantage of better preserving the protein expression levels and metabolic pathway activity of the original liver, including the activation of fatty acid β-oxidation observed in hepatocytes isolated from fasted mice compared to fed mice.

摘要

脂肪酸β-氧化是满足肝脏能量需求的关键代谢途径,并为其他过程(如酮体生成和糖异生)提供底物和辅助因子,这些过程对于维持全身葡萄糖稳态和在禁食状态下支持肝外器官功能至关重要。脂肪酸β-氧化发生在线粒体和过氧化物酶体中,并通过多种机制进行调节,包括脂肪酸的摄取和激活、酶表达水平以及辅助因子(如辅酶 A 和 NAD)的可用性。在测量肝匀浆中脂肪酸β-氧化的测定中,细胞裂解和添加超生理水平的辅助因子掩盖了这些调节机制的影响。此外,匀浆中细胞器的完整性很难控制,并且在不同的制剂之间差异很大。完整原代肝细胞中脂肪酸β-氧化的测量克服了上述缺陷。本协议描述了一种在悬浮于新鲜分离的原代小鼠肝细胞中孵育 C 标记的棕榈酸时测量脂肪酸β-氧化的方法。通过避免数小时到数天的培养,该方法具有更好地保留原始肝脏中蛋白质表达水平和代谢途径活性的优势,包括与喂食小鼠相比,从禁食小鼠中分离的肝细胞中观察到的脂肪酸β-氧化的激活。

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