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Dead-end complex lipid interactions and catalytic mechanism of microsomal glutathione transferase 1 an electron crystallography and mutagenesis investigation

机译:谷胱甘肽转移酶1的死端复合物脂质相互作用和催化机理电子晶体学和诱变研究

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摘要

Microsomal glutathione transferase 1 (MGST1) is a detoxification enzyme belonging to the Membrane Associated Proteins in Eicosanoid and Glutathione Metabolism (MAPEG) superfamily. Here we have used electron crystallography of two-dimensional crystals in order to determine an atomic model of rat MGST1 in a lipid environment. The model comprises 123 of the 155 amino acid residues, two structured phospholipid molecules, two aliphatic chains and one glutathione (GSH) molecule. The functional unit is a homotrimer centered on the crystallographic three-fold axes of the unit cell. The GSH substrate binds in an extended conformation at the interface between two subunits of the trimer supported by new in vitro mutagenesis data. Mutation of Arginine 130 to alanine resulted in complete loss of activity consistent with a role for Arginine 130 in stabilizing the strongly nucleophilic GSH thiolate required for catalysis. Based on the new model and an electron diffraction data set from crystals soaked with trinitrobenzene, that forms a dead-end Meisenheimer complex with GSH, a difference map was calculated. The map reveals side chain movements opening a cavity that defines the second substrate site.
机译:微粒体谷胱甘肽转移酶1(MGST1)是一种排毒酶,属于类二十烷酸和谷胱甘肽代谢(MAPEG)超家族中的膜相关蛋白。在这里,我们已经使用二维晶体的电子晶体学来确定脂质环境中大鼠MGST1的原子模型。该模型包含155个氨基酸残基中的123个,两个结构化的磷脂分子,两个脂族链和一个谷胱甘肽(GSH)分子。功能单元是同质三聚体,其以晶胞的晶体学三重轴为中心。 GSH底物在三聚体的两个亚基之间的界面上以扩展构象结合,新的体外诱变数据支持该界面。精氨酸130突变为丙氨酸导致活性完全丧失,这与精氨酸130在稳定催化所需的强亲核GSH硫醇盐中的作用一致。基于新模型和三硝基苯浸透的晶体的电子衍射数据集,该晶体与GSH形成末端的迈森海默络合物,计算出差异图。该图揭示了侧链运动,从而打开了一个空腔,该空腔定义了第二个基材位置。

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