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KabA 催化途径的快照,KabA 是蜡状芽孢杆菌 UW85 中合成卡那霉素所必需的依赖 PLP 的氨基转移酶。

Snapshots along the catalytic path of KabA, a PLP-dependent aminotransferase required for kanosamine biosynthesis in Bacillus cereus UW85.

机构信息

Department of Chemistry, University of Saskatchewan, Saskatoon, SK S7N 5C9, Canada.

Department of Chemistry, University of Saskatchewan, Saskatoon, SK S7N 5C9, Canada.

出版信息

J Struct Biol. 2021 Jun;213(2):107744. doi: 10.1016/j.jsb.2021.107744. Epub 2021 May 11.

Abstract

Kanosamine is an antibiotic and antifungal monosaccharide. The kanosamine biosynthetic pathway from glucose 6-phosphate in Bacillus cereus UW85 was recently reported, and the functions of each of the three enzymes in the pathway, KabA, KabB and KabC, were demonstrated. KabA, a member of a subclass of the VI family of PLP-dependent aminotransferases, catalyzes the second step in the pathway, generating kanosamine 6-phosphate (K6P) using l-glutamate as the amino-donor. KabA catalysis was shown to be extremely efficient, with a second-order rate constant with respect to K6P transamination of over 10 Ms. Here we report the high-resolution structure of KabA in both the PLP- and PMP-bound forms. In addition, co-crystallization with K6P allowed the structure of KabA in complex with the covalent PLP-K6P adduct to be solved. Co-crystallization or soaking with glutamate or 2-oxoglutarate did not result in crystals with either substrate/product. Reduction of the PLP-KabA complex with sodium cyanoborohydride gave an inactivated enzyme, and crystals of the reduced KabA were soaked with the l-glutamate analog glutarate to mimic the KabA-PLP-l-glutamate complex. Together these four structures give a complete picture of how the active site of KabA recognizes substrates for each half-reaction. The KabA structure is discussed in the context of homologous aminotransferases.

摘要

卡那霉素是一种抗生素和抗真菌单糖。最近报道了蜡样芽胞杆菌 UW85 中葡萄糖 6-磷酸的卡那霉素生物合成途径,并且证明了该途径中三种酶(KabA、KabB 和 KabC)的每个酶的功能。KabA 是 PLP 依赖性转氨酶 VI 家族的一个亚类的成员,催化途径的第二步,使用 l-谷氨酸作为氨基供体生成卡那霉素 6-磷酸(K6P)。KabA 催化被证明是非常有效的,相对于 K6P 转氨的二级速率常数超过 10 Ms。在这里,我们报告了 KabA 在 PLP 和 PMP 结合形式下的高分辨率结构。此外,与 K6P 的共结晶允许解决 KabA 与共价 PLP-K6P 加合物复合物的结构。与谷氨酸或 2-氧代戊二酸共结晶或浸泡均未导致任一底物/产物的晶体形成。用氰基硼氢化钠还原 PLP-KabA 复合物产生了失活的酶,并用 l-谷氨酸类似物戊二酸盐浸泡还原的 KabA 以模拟 KabA-PLP-l-谷氨酸复合物。这四个结构共同提供了 KabA 活性位点如何识别每个半反应的底物的完整图景。KabA 结构在同源转氨酶的背景下进行了讨论。

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