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肠杆菌素生物合成中间体2,3 - 二羟基苯甲酸是大肠杆菌异分支酸酶EntB的竞争性抑制剂。

The enterobactin biosynthetic intermediate 2,3-dihydroxybenzoic acid is a competitive inhibitor of the Escherichia coli isochorismatase EntB.

作者信息

Bin Xue, Pawelek Peter D

机构信息

Department of Chemistry and Biochemistry, Concordia University, Montreal, Quebec, Canada.

出版信息

Protein Sci. 2025 Jun;34(6):e70160. doi: 10.1002/pro.70160.

DOI:10.1002/pro.70160
PMID:40400396
Abstract

The Escherichia coli enterobactin biosynthetic protein EntB is a bifunctional enzyme that catalyzes hydrolysis of isochorismate via its N-terminal isochorismatase (IC) domain, and then transfers phosphopantetheinylated 2,3-DHB to EntF via the EntB C-terminal aryl carrier protein (ArCP) domain. Here we used a fluorescence anisotropy binding assay to investigate the ability of 2,3-DHB to bind to enzymes in the DHB synthetic arm of the pathway. We found that 2,3-DHB binds to EntE as a natural substrate with high affinity (K = 0.54 μM). Furthermore, apo-EntB was found to bind to 2,3-DHB with moderate affinity (K = 8.95 μM), despite the fact that this intermediate is neither a substrate nor a product of EntB. Molecular docking simulations predicted a top-ranked ensemble in which 2,3-DHB is bound at the isochorismatase active site of apo-EntB. Steady-state coupled enzymatic assays revealed that 2,3-DHB is a competitive inhibitor of apo-EntB isochorismatase activity (K ~ 200 μM), consistent with modeling predictions. Monitoring the EntC-EntB coupled reaction in real time via isothermal titration microcalorimetry confirmed that EntB was required to drive the EntC reaction toward isochorismate formation. Furthermore, addition of 2,3-DHB to the ITC-monitored reaction resulted in a suppression of integrated reaction heats, consistent with our observation that the molecule acts as a competitive inhibitor of EntB. Finally, we found that 2,3-DHB lowered the efficiency of EntC-EntB isochorismate channeling by approximately 70%, consistent with steric blockage of the isochorismatase active site by bound 2,3-DHB. Given its inhibitory properties, we hypothesize that 2,3-DHB plays a regulatory role in feedback inhibition in order to maintain iron homeostasis upon intracellular accumulation of sufficient ferric enterobactin.

摘要

大肠杆菌肠杆菌素生物合成蛋白EntB是一种双功能酶,它通过其N端异分支酸酶(IC)结构域催化异分支酸的水解,然后通过EntB的C端芳基载体蛋白(ArCP)结构域将磷酸泛酰巯基乙胺化的2,3 -二羟基苯甲酸(2,3-DHB)转移至EntF。在此,我们使用荧光各向异性结合测定法来研究2,3-DHB与该途径中二羟基苯甲酸合成臂中的酶结合的能力。我们发现,2,3-DHB作为天然底物以高亲和力(K = 0.54 μM)与EntE结合。此外,尽管该中间体既不是EntB的底物也不是其产物,但发现脱辅基EntB以中等亲和力(K = 8.95 μM)与2,3-DHB结合。分子对接模拟预测了一个排名靠前的组合,其中2,3-DHB结合在脱辅基EntB的异分支酸酶活性位点。稳态偶联酶促测定表明,2,3-DHB是脱辅基EntB异分支酸酶活性的竞争性抑制剂(K ~ 200 μM),这与模型预测一致。通过等温滴定量热法实时监测EntC-EntB偶联反应证实,EntB是驱动EntC反应生成异分支酸所必需的。此外,向等温滴定量热法监测的反应中添加2,3-DHB导致积分反应热受到抑制,这与我们观察到该分子作为EntB的竞争性抑制剂的结果一致。最后,我们发现2,3-DHB使EntC-EntB异分支酸通道化效率降低了约70%,这与结合的2,3-DHB对异分支酸酶活性位点的空间位阻一致。鉴于其抑制特性,我们推测2,3-DHB在反馈抑制中发挥调节作用,以便在细胞内积累足够的铁载体肠杆菌素时维持铁稳态。

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Evidence of an intracellular interaction between the Escherichia coli enzymes EntC and EntB and identification of a potential electrostatic channeling surface.
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