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使用重组猪电子传递黄素蛋白的酰基辅酶 A 脱氢酶微孔板活性测定法。

An acyl-CoA dehydrogenase microplate activity assay using recombinant porcine electron transfer flavoprotein.

机构信息

Department of Pediatrics, Division of Medical Genetics, University of Pittsburgh School of Medicine, Children's Hospital of Pittsburgh, 4401 Penn Avenue, Pittsburgh, PA, 15224, USA.

Department of Pediatrics, Division of Medical Genetics, University of Pittsburgh School of Medicine, Children's Hospital of Pittsburgh, 4401 Penn Avenue, Pittsburgh, PA, 15224, USA.

出版信息

Anal Biochem. 2019 Sep 15;581:113332. doi: 10.1016/j.ab.2019.06.003. Epub 2019 Jun 10.

Abstract

Acyl-CoA dehydrogenases (ACADs) play key roles in the mitochondrial catabolism of fatty acids and branched-chain amino acids. All nine characterized ACAD enzymes use electron transfer flavoprotein (ETF) as their redox partner. The gold standard for measuring ACAD activity is the anaerobic ETF fluorescence reduction assay, which follows the decrease of pig ETF fluorescence as it accepts electrons from an ACAD in vitro. Although first described 35 years ago, the assay has not been widely used due to the need to maintain an anaerobic assay environment and to purify ETF from pig liver mitochondria. Here, we present a method for expressing recombinant pig ETF in E coli and purifying it to homogeneity. The recombinant protein is virtually pure after one chromatography step, bears higher intrinsic fluorescence than the native enzyme, and provides enhanced activity in the ETF fluorescence reduction assay. Finally, we present a simplified protocol for removing molecular oxygen that allows adaption of the assay to a 96-well plate format. The availability of recombinant pig ETF and the microplate version of the ACAD activity assay will allow wide application of the assay for both basic research and clinical diagnostics.

摘要

酰基辅酶 A 脱氢酶(ACADs)在脂肪酸和支链氨基酸的线粒体分解代谢中发挥关键作用。所有九种已鉴定的 ACAD 酶都使用电子转移黄素蛋白(ETF)作为其氧化还原伴侣。测量 ACAD 活性的金标准是厌氧 ETF 荧光还原测定法,该方法通过体外接受来自 ACAD 的电子来跟踪猪 ETF 荧光的减少。尽管该测定法 35 年前首次描述,但由于需要维持厌氧测定环境并从猪肝线粒体中纯化 ETF,因此尚未广泛使用。在这里,我们提出了一种在大肠杆菌中表达重组猪 ETF 并将其纯化至均相的方法。经过一步层析,该重组蛋白几乎是纯的,比天然酶具有更高的固有荧光,并在 ETF 荧光还原测定中提供了增强的活性。最后,我们提出了一种简化的去除分子氧的方案,该方案允许将测定法适用于 96 孔板格式。重组猪 ETF 和微板版 ACAD 活性测定法的出现将使该测定法在基础研究和临床诊断中得到广泛应用。

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