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Homogeneous and heterogeneous dynamics in native and denatured bovine serum albumin

机译:天然和变性牛血清白蛋白的同质和异构动态

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A characteristic property of unfolded and disordered proteins is their high molecular flexibility, which enables the exploration of a large conformational space. We present neutron scattering experiments on the dynamics of denatured and native folded bovine serum albumin (BSA) in solution. Global protein diffusion and internal macromolecular dynamics were measured using quasielastic neutron time-of-flight and backscattering spectroscopy on the picosecond to nanosecond time-and Angstrom length-scale. Internal protein dynamics were analysed in a first approach using stretched exponential functions. In denatured BSA predominantly slow heterogeneous dynamics dominates the observed macromolecular motions. Reduction of disulphide bridges in denatured BSA does not significantly alter the visible motions. In native folded BSA fast homogeneous dynamics and slow heterogeneous dynamics were observed. In an alternative data analysis approach, internal protein dynamics was interpreted using the analytical model of the overdamped Brownian oscillator, which allowed us to extract mean square displacements of protein internal dynamics and the fraction of hydrogen atoms participating in the observed motions. Our results demonstrate that denaturation modifies the physical nature of internal protein dynamics significantly as compared to the native folded structure.
机译:展开和无序蛋白质的特征性是它们的高分子柔性,能够探索大构象空间。我们对溶液中变性和天然折叠牛血清白蛋白(BSA)的动态进行节奏散射实验。使用Quasielast中的中子飞行时间和背散射光谱法测量全局蛋白质扩散和内部大分子动力学在PICOSECOND上以纳秒时间和宽度长度级。使用拉伸指数函数的第一种方法分析内部蛋白质动态。在变性BSA中,主要是缓慢的异构动态主导观察到的大分子运动。减少变性BSA中的二硫桥不会显着改变可见运动。在本地折叠BSA中,观察到快速均匀的动态和缓慢的异构动态。在替代数据分析方法中,使用覆盖褐色振荡器的分析模型来解释内部蛋白质动态,这使我们允许我们提取蛋白质内部动力学的均方位移和参与观察到的运动的氢原子的级分。我们的结果表明,与天然折叠结构相比,变性显着改变内部蛋白质动力学的物理性质。

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