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参与鱼腥藻毒素-a 和同鱼腥藻毒素-a 生物合成的脯氨酰-酰基载体蛋白氧化酶反应机制的研究进展。

Insights into the reaction mechanism of the prolyl-acyl carrier protein oxidase involved in anatoxin-a and homoanatoxin-a biosynthesis.

机构信息

Laboratoire Charles Friedel, Chimie ParisTech, ENSCP, 11 rue Pierre et Marie Curie, 75231 Paris Cedex 05, France.

出版信息

Biochemistry. 2011 Aug 23;50(33):7184-97. doi: 10.1021/bi200892a. Epub 2011 Jul 27.

DOI:10.1021/bi200892a
PMID:21786780
Abstract

Anatoxin-a and homoanatoxin-a are two potent cyanobacterial neurotoxins. We recently reported the identification of the gene cluster responsible for the biosynthesis of these toxins as well as the in-vitro reconstitution of the first steps of this biosynthesis. We now report experimental evidence supporting the proposed reaction mechanism of AnaB, a flavoprotein homologous to acyl-CoA dehydrogenase. AnaB catalyzes the two-electron oxidation of prolyl-AnaD, which is proline linked to the acyl carrier protein holo-AnaD, to dehydroprolyl-AnaD using oxygen as the second substrate. AnaB is thus an oxidase. By using liquid chromatography coupled to tandem mass spectrometry (LC-MS/MS), we have identified and characterized dehydroprolyl-AnaD, the AnaB product. We estimated an apparent catalytic constant of 1 min(-1) for AnaB catalysis. We synthesized several deuterium-labeled prolines and enzymatically transformed them into their corresponding prolyl-AnaD. These deuterium-labeled prolyl-AnaDs were oxidized in the presence of AnaB, and the deuterium labeling in the remaining substrate and in the product was determined by LC-MS/MS. The data supported a reaction mechanism starting with a rapid enolization followed by a slow oxidation to give the conjugated imine, which in turn was isomerized to pyrroline-5-carboxyl-AnaD. We also showed that cis- and trans-4-fluoro-L-prolyl-AnaD and 3,4-dehydro-L-prolyl-AnaD were transformed into pyrrole-2-carboxyl-AnaD by AnaB. Thus, the 4-fluoro-analogues experienced a β-elimination supporting the AnaB-catalyzed aza-allylic isomerization. We identified by sequence alignment the AnaB active site base, Glu244. We produced, purified, and characterized the E244A AnaB mutant, which is inactive, supporting the catalytic role of E244 as a base.

摘要

石房蛤毒素-a 和同石房蛤毒素-a 是两种强效的蓝藻神经毒素。我们最近报道了负责这些毒素生物合成的基因簇的鉴定,以及该生物合成的第一步的体外重建。我们现在报告了支持 AnaB(一种与酰基辅酶 A 脱氢酶同源的黄素蛋白)提议的反应机制的实验证据。AnaB 催化脯氨酸与酰基载体蛋白全同型 AnaD 连接的 prolyl-AnaD 的两个电子氧化,使用氧作为第二个底物将其转化为 dehydroprolyl-AnaD。因此,AnaB 是一种氧化酶。通过使用液相色谱与串联质谱(LC-MS/MS),我们已经鉴定并表征了 AnaB 产物 dehydroprolyl-AnaD。我们估计 AnaB 催化的表观催化常数为 1 min(-1)。我们合成了几种氘标记的脯氨酸,并通过酶促转化将它们转化为相应的 prolyl-AnaD。这些氘标记的 prolyl-AnaD 在 AnaB 的存在下被氧化,并用 LC-MS/MS 确定剩余底物和产物中的氘标记。数据支持从快速烯醇化开始的反应机制,然后是缓慢氧化生成共轭亚胺,接着是互变异构化得到吡咯啉-5-羧酸-AnaD。我们还表明 cis- 和 trans-4-氟-L-脯氨酸-AnaD 和 3,4-脱氢-L-脯氨酸-AnaD 被 AnaB 转化为吡咯-2-羧酸-AnaD。因此,4-氟类似物经历β-消除,支持 AnaB 催化的氮杂烯丙基异构化。我们通过序列比对鉴定了 AnaB 的活性位点碱基,Glu244。我们生产、纯化并表征了无活性的 E244A AnaB 突变体,这支持了 E244 作为碱基的催化作用。

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