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细菌 N-去甲基酶复合物催化咖啡因降解的结构与机制研究。

Structural and Mechanistic Insights into Caffeine Degradation by the Bacterial N-Demethylase Complex.

机构信息

Department of Life Sciences, Korea University, 145 Anam-ro, Seongbuk-gu, Seoul 02841, Republic of Korea.

Department of Chemical and Biological Engineering, The University of Alabama, Tuscaloosa, AL 35487, USA.

出版信息

J Mol Biol. 2019 Sep 6;431(19):3647-3661. doi: 10.1016/j.jmb.2019.08.004. Epub 2019 Aug 11.

DOI:10.1016/j.jmb.2019.08.004
PMID:31412262
Abstract

Caffeine, found in many foods, beverages, and pharmaceuticals, is the most used chemical compound for mental alertness. It is originally a natural product of plants and exists widely in environmental soil. Some bacteria, such as Pseudomonas putida CBB5, utilize caffeine as a sole carbon and nitrogen source by degrading it through sequential N-demethylation catalyzed by five enzymes (NdmA, NdmB, NdmC, NdmD, and NdmE). The environmentally friendly enzymatic reaction products, methylxanthines, are high-value biochemicals that are used in the pharmaceutical and cosmetic industries. However, the structures and biochemical properties of bacterial N-demethylases remain largely unknown. Here, we report the structures of NdmA and NdmB, the initial N- and N-specific demethylases, respectively. Reverse-oriented substrate bindings were observed in the substrate-complexed structures, offering methyl position specificity for proper N-demethylation. For efficient sequential degradation of caffeine, these enzymes form a unique heterocomplex with 3:3 stoichiometry, which was confirmed by enzymatic assays, fluorescent labeling, and small-angle x-ray scattering. The binary structure of NdmA with the ferredoxin domain of NdmD, which is the first structural information for the plant-type ferredoxin domain in a complex state, was also determined to better understand electron transport during N-demethylation. These findings broaden our understanding of the caffeine degradation mechanism by bacterial enzymes and will enable their use for industrial applications.

摘要

咖啡因存在于许多食物、饮料和药物中,是提高精神警觉性最常用的化学物质。它最初是植物的天然产物,广泛存在于环境土壤中。一些细菌,如假单胞菌(Pseudomonas putida CBB5),通过五种酶(NdmA、NdmB、NdmC、NdmD 和 NdmE)的顺序 N-去甲基化作用来降解咖啡因,将其作为唯一的碳氮源加以利用。环境友好型的酶促反应产物,即甲基黄嘌呤,是高价值的生化物质,用于制药和化妆品行业。然而,细菌 N-去甲基酶的结构和生化特性在很大程度上仍然未知。在这里,我们报告了 NdmA 和 NdmB 的结构,它们分别是最初的 N-和 N-特异性去甲基酶。在与底物结合的结构中观察到反向定向的底物结合,为正确的 N-去甲基化提供了甲基位置特异性。为了高效地顺序降解咖啡因,这些酶以 3:3 的化学计量比形成独特的杂合复合物,这通过酶促测定、荧光标记和小角 X 射线散射得到了证实。还确定了 NdmA 与 NdmD 的铁氧还蛋白结构域的二元结构,这是首次在复合物状态下确定植物型铁氧还蛋白结构域的结构信息,以便更好地理解 N-去甲基化过程中的电子传递。这些发现拓宽了我们对细菌酶降解咖啡因机制的理解,并将使它们能够用于工业应用。

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