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鸟苷 5'-单磷酸合成酶的底物激活和构象动力学。

Substrate activation and conformational dynamics of guanosine 5'-monophosphate synthetase.

机构信息

Department of Medicinal Chemistry and Molecular Pharmacology, Purdue University , West Lafayette, Indiana 47907, United States.

出版信息

Biochemistry. 2013 Aug 6;52(31):5225-35. doi: 10.1021/bi3017075. Epub 2013 Jul 23.

Abstract

Glutamine amidotransferases catalyze the amination of a wide range of molecules using the amide nitrogen of glutamine. The family provides numerous examples for study of multi-active-site regulation and interdomain communication in proteins. Guanosine 5'-monophosphate synthetase (GMPS) is one of three glutamine amidotransferases in de novo purine biosynthesis and is responsible for the last step in the guanosine branch of the pathway, the amination of xanthosine 5'-monophosphate (XMP). In several amidotransferases, the intramolecular path of ammonia from glutamine to substrate is understood; however, the crystal structure of GMPS only hinted at the details of such transfer. Rapid kinetics studies provide insight into the mechanism of the substrate-induced changes in this complex enzyme. Rapid mixing of GMPS with substrates also manifests absorbance changes that report on the kinetics of formation of a reactive intermediate as well as steps in the process of rapid transfer of ammonia to this intermediate. Isolation and use of the adenylylated nucleotide intermediate allowed the study of the amido transfer reaction distinct from the ATP-dependent reaction. Changes in intrinsic tryptophan fluorescence upon mixing of enzyme with XMP suggest a conformational change upon substrate binding, likely the ordering of a highly conserved loop in addition to global domain motions. In the GMPS reaction, all forward rates before product release appear to be faster than steady-state turnover, implying that release is likely rate-limiting. These studies establish the functional role of a substrate-induced conformational change in the GMPS catalytic cycle and provide a kinetic context for the formation of an ammonia channel linking the distinct active sites.

摘要

谷氨酰胺酰胺转移酶利用谷氨酰胺的酰胺氮催化广泛的分子胺化。该家族为研究多活性位点调节和蛋白质的域间通讯提供了许多例子。鸟苷 5'-单磷酸合酶 (GMPS) 是从头嘌呤生物合成中的三种谷氨酰胺酰胺转移酶之一,负责途径中鸟苷分支的最后一步,即黄苷 5'-单磷酸 (XMP) 的胺化。在几种酰胺转移酶中,已了解到从谷氨酰胺到底物的氨的分子内途径;然而,GMPS 的晶体结构仅暗示了这种转移的细节。快速动力学研究为了解该复杂酶中底物诱导变化的机制提供了线索。GMPS 与底物的快速混合也表现出吸光度变化,这些变化报告了活性中间产物形成的动力学以及将氨快速转移到该中间产物的过程中的步骤。腺苷酰化核苷酸中间产物的分离和使用允许研究与 ATP 依赖性反应不同的酰胺转移反应。酶与 XMP 混合时固有色氨酸荧光的变化表明在底物结合时发生构象变化,可能是除了全局结构域运动之外,还对高度保守的环进行了有序排列。在 GMPS 反应中,在产物释放之前的所有正向速率似乎都比稳态周转率快,这意味着释放可能是限速步骤。这些研究确立了底物诱导构象变化在 GMPS 催化循环中的功能作用,并为形成连接不同活性位点的氨通道提供了动力学背景。

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