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艰难梭菌 2-羟基异己酰基辅酶 A 脱水酶与其激活剂复合物的稳定化,通过四氟化铝-腺苷二磷酸实现。

A complex of 2-hydroxyisocaproyl-coenzyme A dehydratase and its activator from Clostridium difficile stabilized by aluminium tetrafluoride-adenosine diphosphate.

机构信息

Fachbereich Biologie, Philipps Universität, 35032 Marburg, Germany.

出版信息

Chemphyschem. 2010 Apr 26;11(6):1307-12. doi: 10.1002/cphc.200900876.

DOI:10.1002/cphc.200900876
PMID:20146278
Abstract

The dehydration of 2-hydroxyisocaproyl-CoA to isocaprenoyl-CoA is the chemically most demanding step in the reduction of leucine to isocaproate by Clostridium difficile, because the beta-hydrogen of the substrate is not acidic (pK(a) ca. 40). A two-component system, composed of a homodimeric activator and an heterodimeric dehydratase, catalyses this unusual alpha,beta-elimination of water. The reduced activator transfers an electron from its 4Fe-4S cluster to that of the dehydratase in an ATP-dependent manner, similar to the iron protein of nitrogenase. Here we show that AlF(4)(-) x ADP traps the interaction of the activator with the dehydratase by forming a stable complex containing 1.0 mol homodimeric activator, 1.0 mol heterodimeric dehydratase and 1.2 mol ADP. The complex (148 kDa) was isolated by size exclusion chromatography, affinity chromatography using the Strep-tag at the activator, or most conveniently by ultrafiltration (100 kDa cut off membrane). Kinetic and EPR-spectroscopic experiments revealed that the complex formation proceeds much slower than the activation but in an almost irreversible manner. The isolated complex is devoid of any activity, because the dehydratase is in the oxidized form whereas the activator remains in the reduced state due to the presence of dithionite.

摘要

艰难梭菌将 2-羟基异己酰辅酶 A 脱水为异己酰辅酶 A 的过程是将亮氨酸还原为异己酸的所有步骤中化学要求最高的一步,因为底物的β-氢并非酸性(pK(a) 约为 40)。由一个同二聚体激活剂和一个异二聚体脱水酶组成的两个组件系统催化这种不寻常的α,β-消除水的反应。还原的激活剂以依赖于 ATP 的方式将电子从其 4Fe-4S 簇转移到脱水酶的电子上,类似于氮酶的铁蛋白。在这里,我们表明 AlF(4)(-) x ADP 通过形成含有 1.0 mol 同二聚体激活剂、1.0 mol 异二聚体脱水酶和 1.2 mol ADP 的稳定复合物来捕获激活剂与脱水酶的相互作用。该复合物(148 kDa)通过大小排阻色谱法、使用激活剂上的 Strep 标签的亲和色谱法或最方便的超滤(100 kDa 截止膜)进行分离。动力学和 EPR 光谱实验表明,复合物的形成速度远低于激活速度,但几乎是不可逆的。由于存在连二亚硫酸盐,分离出的复合物没有任何活性,因为脱水酶处于氧化形式,而激活剂仍然处于还原状态。

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