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一种新型的 ATP 柠檬酸裂解酶的直接均相测定法。

A novel direct homogeneous assay for ATP citrate lyase.

机构信息

Department of Metabolic Research, Research and Development, Bristol-Myers Squibb Company, Princeton, NJ 08543-5400, USA.

出版信息

J Lipid Res. 2009 Oct;50(10):2131-5. doi: 10.1194/jlr.D900008-JLR200. Epub 2009 Mar 12.

Abstract

ATP citrate lyase (ACL) is a cytosolic enzyme that catalyzes the synthesis of acetyl-CoA and oxaloacetate using citrate, CoA, and ATP as substrates and Mg(2+) as a necessary cofactor. The ACL-dependent synthesis of acetyl-CoA is thought to be an essential step for the de novo synthesis of fatty acids and cholesterol. For this reason, inhibition of ACL has been pursued as a strategy to treat dyslipidemia and obesity. Traditionally, ACL enzyme activity is measured indirectly by coupling to enzymes such as malate dehydrogenase or chloramphenicol acetyl transferase. In this report, however, we describe a novel procedure to directly measure ACL enzyme activity. We first identified a convenient method to specifically detect [(14)C]acetyl-CoA without detecting [(14)C]citrate by MicroScint-O. Using this detection system, we devised a simple, direct, and homogeneous ACL assay in 384-well plate format that is suitable for high-throughput screening. The current assay consists of 1) incubation of ACL enzyme with [(14)C]citrate and other substrates/cofactors CoA, ATP, and Mg(2+), 2) EDTA quench, 3) addition of MicroScint-O, the agent that specifically detects product [(14)C]acetyl-CoA, and 4) detection of signal by TopCount. This unique ACL assay may provide more efficient identification of new ACL inhibitors and allow detailed mechanistic characterization of ACL/inhibitor interactions.

摘要

三磷酸腺苷柠檬酸裂解酶(ACL)是一种胞质酶,可利用柠檬酸、CoA、ATP 作为底物,以及 Mg(2+)作为必需辅助因子,催化乙酰 CoA 和草酰乙酸的合成。据认为,ACL 依赖性乙酰 CoA 的合成是脂肪酸和胆固醇从头合成的一个必要步骤。出于这个原因,抑制 ACL 已被作为治疗血脂异常和肥胖的一种策略进行研究。传统上,ACL 酶活性通过与苹果酸脱氢酶或氯霉素乙酰转移酶等酶偶联来间接测量。然而,在本报告中,我们描述了一种直接测量 ACL 酶活性的新方法。我们首先通过 MicroScint-O 确定了一种方便的方法,可特异性地检测 [(14)C]乙酰 CoA,而不会检测 [(14)C]柠檬酸。使用该检测系统,我们设计了一种简单、直接、均相的 384 孔板格式的 ACL 测定法,适用于高通量筛选。目前的测定法包括:1)将 ACL 酶与 [(14)C]柠檬酸和其他底物/辅助因子 CoA、ATP 和 Mg(2+)孵育;2)EDTA 淬灭;3)加入 MicroScint-O,该试剂可特异性地检测产物 [(14)C]乙酰 CoA;4)通过 TopCount 检测信号。这种独特的 ACL 测定法可能会更有效地鉴定新的 ACL 抑制剂,并允许对 ACL/抑制剂相互作用进行详细的机制表征。

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