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Enhanced picture of protein-folding intermediates using organic solvents in H/D exchange and quench-flow experiments

机译:在H / D交换和猝灭流动实验中使用有机溶剂的蛋白质折叠中间体的增强图片

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摘要

Hydrogen/deuterium exchange followed by trapping of the labeled species in the aprotic solvent DMSO has been used to elucidate structure in both the burst-phase molten globule-folding intermediate of apomyoglobin and in an equilibrium intermediate that models the kinetic intermediate. Precise estimates can be made of exchange times in an interrupted exchange-out experiment at pH 4 followed by analysis in DMSO solution, giving extensive sequence-specific information about the structure of the equilibrium intermediate. In addition, the use of DMSO as a solvent for NMR measurements after quench-flow pH-pulse labeling experiments gives a greatly increased data set for the elucidation of the kinetic folding pathway. Interestingly, differences are observed in some regions of apomyoglobin between the equilibrium and kinetic intermediates. These differences are quantitative rather than qualitative; that is, the overall patterns of labeling and secondary structure formation remain similar between the two species. However, local differences are observed, which probably reflect the difference in the solution conditions for the equilibrium experiment (pH 4) vs. the kinetic experiment (pH 6) and the change in the status of the stabilizing hydrogen bond between the side chains of His-24 and His-119.
机译:氢/氘交换,然后在非质子传递溶剂DMSO中捕获标记物质,已被用于阐明肌红蛋白爆裂相熔融球状折叠中间体和模拟动力学中间体的平衡中间体中的结构。可以在pH 4的中断交换实验中精确估算交换时间,然后在DMSO溶液中进行分析,从而获得有关平衡中间体结构的大量序列特定信息。此外,在淬灭流pH脉冲标记实验后,使用DMSO作为NMR测量的溶剂可大大增加阐明动力学折叠途径的数据集。有趣的是,在平衡肌蛋白和动力学中间体之间的磷肌红蛋白的某些区域观察到差异。这些差异是定量的,而不是定性的。也就是说,两种物种之间标记和二级结构形成的总体模式保持相似。但是,观察到局部差异,这可能反映了平衡实验(pH 4)与动力学实验(pH 6)的溶液条件差异以及His侧链之间稳定氢键状态的变化。 -24和His-119。

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