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脂肪酰辅酶A脱氢酶与脂肪酰辅酶A氧化酶的结构-功能相关性

Structure-function correlation of fatty acyl-CoA dehydrogenase and fatty acyl-CoA oxidase.

作者信息

Rojas C, Schmidt J, Lee M Y, Gustafson W G, McFarland J T

出版信息

Biochemistry. 1985 Jun 4;24(12):2947-54. doi: 10.1021/bi00333a021.

DOI:10.1021/bi00333a021
PMID:4040392
Abstract

We have employed a new pseudosubstrate, beta-(2-furyl)propionyl coenzyme A (FPCoA), to study the functional properties of two enzymes, fatty acyl-CoA dehydrogenase from porcine liver and fatty acyl-CoA oxidase from Candida tropicalis, involved in the oxidation of fatty acids. Previous studies from our laboratory have shown that the dehydrogenase exhibits oxidase activity at the rate of dissociation of the product charge-transfer complex. This raises the question of the difference in functionality between these two flavoproteins. To investigate these differences, we have compared the pH dependence of product formation, the isotope effects using tetradeuterio-FPCoA, and the spectral properties and chemical reactivity of the product charge-transfer complexes formed with the two enzymes. The pH dependencies of the reaction of FPCoA with electron-transfer flavoprotein (ETF) for the dehydrogenase and of the reaction of FPCoA with O2 for the oxidase are quite similar. Both reactions proceed more rapidly at basic pH values while substrate binds more tightly at acidic pH values. These data for both enzymes are consistent with a mechanism in which enzyme is involved in protonation of the carbonyl group of substrate followed by base-catalyzed removal of the C-2 proton from substrate. The C-2 anion of substrate may then serve as the active species in reduction of enzyme-bound flavin. The deuterium isotope effects for both enzyme systems are primary across the entire pH range, assuring that the chemically important step of substrate oxidation is rate limiting in these steady-state kinetic experiments. The two enzymes differ in the chemical reactivity of their product charge-transfer complexes.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

我们使用了一种新的假底物,β-(2-呋喃基)丙酰辅酶A(FPCoA),来研究两种参与脂肪酸氧化的酶的功能特性,即猪肝中的脂肪酰辅酶A脱氢酶和热带假丝酵母中的脂肪酰辅酶A氧化酶。我们实验室之前的研究表明,该脱氢酶在产物电荷转移复合物解离速率下表现出氧化酶活性。这就引发了这两种黄素蛋白功能差异的问题。为了研究这些差异,我们比较了产物形成的pH依赖性、使用四氘代FPCoA的同位素效应,以及与这两种酶形成的产物电荷转移复合物的光谱特性和化学反应性。FPCoA与脱氢酶的电子传递黄素蛋白(ETF)反应的pH依赖性,以及FPCoA与氧化酶的O2反应的pH依赖性非常相似。两种反应在碱性pH值下进行得更快,而底物在酸性pH值下结合更紧密。这两种酶的这些数据都与一种机制一致,即酶参与底物羰基的质子化,随后碱催化从底物上去除C-2质子。底物的C-2阴离子然后可以作为还原酶结合黄素的活性物种。在整个pH范围内,两种酶系统的氘同位素效应都是一级的,这确保了在这些稳态动力学实验中,底物氧化的化学重要步骤是限速步骤。这两种酶的产物电荷转移复合物的化学反应性不同。(摘要截断于250字)

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