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Construction of a 3D model of nattokinase, a novel fibrinolytic enzyme from Bacillus natto A novel nucleophilic catalytic mechanism for nattokinase

机译:纳豆芽孢杆菌新型纤溶酶纳豆激酶3D模型的建立纳豆激酶的新型亲核催化机理

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A three-dimensional structural model of nattokinase (NK) from Bacillus natto was constructed by homology modeling. High-resolution X-ray structures of Subtilisin BPN' (SB), Subtilisin Carlsberg (SC), Subtilisin E (SE) and Subtilisin Savinase (SS), four proteins with sequential, structural and functional homology were used as templates. Initial models of NK were built by MODELLER and analyzed by the PROCHECK programs. The best quality model was chosen for further refinement by constrained molecular dynamics simulations. The overall quality of the refined model was evaluated. The refined model NKC1 was analyzed by different protein analysis programs including PROCHECK for the evaluation of Ramachandran plot quality, PROSA for testing interaction energies and WHATIF for the calculation of packing quality. This structure was found to be satisfactory and also stable at room temperature as demonstrated by a 300 ps long unconstrained molecular dynamics (MD) simulation. Further docking analysis promoted the coming of a new nucleophilic catalytic mechanism for NK, which is induced by attacking of hydroxyl rich in catalytic environment and locating of S221.
机译:通过同源性建模,构建了纳豆芽孢杆菌的纳豆激酶(NK)的三维结构模型。枯草杆菌蛋白酶BPN'(SB),枯草杆菌蛋白酶Carlsberg(SC),枯草杆菌蛋白酶E(SE)和枯草杆菌蛋白酶Savinase(SS)的高分辨率X射线结构,具有顺序,结构和功能同源性的四种蛋白质用作模板。 NK的初始模型是由MODELLER建立的,并由PROCHECK程序进行了分析。通过约束分子动力学模拟,选择了最佳质量模型进行进一步优化。评价了改进模型的整体质量。精制的模型NKC1通过不同的蛋白质分析程序进行了分析,包括PROCHECK(用于评估Ramachandran地块质量),PROSA(用于测试相互作用能)和WHATIF(用于计算包装质量)。通过300 ps长的不受约束的分子动力学(MD)模拟证明,该结构令人满意,并且在室温下也很稳定。进一步的对接分析促进了NK亲核催化新机制的出现,该机制是由催化环境中富含羟基的羟基攻击和S221的定位引起的。

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