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Dynamics at the protein-water interface from 17O spin relaxation in deeply supercooled solutions

机译:在深度过冷溶液中17O自旋弛豫的蛋白质 - 水界面的动力学

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摘要

Most of the decisive molecular events in biology take place at the protein-water interface. The dynamical properties of the hydration layer are therefore of fundamental importance. To characterize the dynamical heterogeneity and rotational activation energy in the hydration layer, we measured the 17O spin relaxation rate in dilute solutions of three proteins in a wide temperature range extending down to 238 K. We find that the rotational correlation time can be described by a power-law distribution with exponent 2.1 – 2.3. Except for a small fraction of secluded hydration sites, the dynamic perturbation in the hydration layer is the same for all proteins and does not differ in any essential way from the hydration shell of small organic solutes. In both cases, the dynamic perturbation factor is less than 2 at room temperature and exhibits a maximum near 260 K. This maximum implies that, at low temperatures, the rate of water molecule rotation has a weaker temperature dependence in the hydration layer than in bulk water. We attribute this difference to the temperature-independent constraints that the protein surface imposes on the water H-bond network. The free hydration layer studied here differs qualitatively from confined water in solid protein powder samples.
机译:生物学中大多数决定性的分子事件发生在蛋白质-水的界面上。因此,水合层的动力学性质至关重要。为了表征水合层中的动力学非均质性和旋转活化能,我们测量了在低至238 K的宽温度范围内三种蛋白质的稀溶液中的17O自旋弛豫速率。我们发现旋转相关时间可以用幂律分布,指数为2.1 – 2.3。除了一小部分僻静的水合位点外,水合层中的动态扰动对于所有蛋白质都是相同的,并且与小有机溶质的水合壳没有任何本质上的区别。在这两种情况下,室温下的动态扰动因子均小于2,并且在260 K附近表现出最大值。该最大值表明,在低温下,水分子在水化层中的旋转速率对温度的依赖性比在体中弱。水。我们将此差异归因于蛋白质表面强加于水H键网络上的温度无关约束。此处研究的游离水合层在质量上与固体蛋白粉样品中的受限水不同。

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