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Coupled protein domain motion in Taq polymerase revealed by neutron spin-echo spectroscopy

机译:Taq聚合酶中的中子自旋回波光谱显示耦合的蛋白质结构域运动。

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摘要

Long-range conformational changes in proteins are ubiquitous in biology for the transmission and amplification of signals; such conformational changes can be triggered by small-amplitude, nanosecond protein domain motion. Understanding how conformational changes are initiated requires the characterization of protein domain motion on these timescales and on length scales comparable to protein dimensions. Using neutron spin-echo spectroscopy (NSE), normal mode analysis, and a statistical-mechanical framework, we reveal overdamped, coupled domain motion within DNA polymerase I from Thermus aquaticus (Taq polymerase). This protein utilizes correlated domain dynamics over 70 Å to coordinate nucleotide synthesis and cleavage during DNA synthesis and repair. We show that NSE spectroscopy can determine the domain mobility tensor, which determines the degree of dynamical coupling between domains. The mobility tensor defines the domain velocity response to a force applied to it or to another domain, just as the sails of a sailboat determine its velocity given the applied wind force. The NSE results provide insights into the nature of protein domain motion that are not appreciated by conventional biophysical techniques.
机译:蛋白质的远距离构象变化在生物学中普遍存在,用于信号的传递和放大。这种构象变化可以由小幅度的纳秒级蛋白质结构域运动触发。了解构象变化是如何开始的,要求在这些时间尺度和与蛋白质尺度可比的长度尺度上表征蛋白质结构域运动。使用中子自旋回波光谱(NSE),正常模式分析和统计力学框架,我们揭示了水生栖热菌(Taq聚合酶)的DNA聚合酶I内过度阻尼的耦合域运动。该蛋白利用70Å以上的相关域动态来协调DNA合成和修复过程中的核苷酸合成和裂解。我们表明,NSE光谱学可以确定域迁移率张量,而张量决定了域之间的动态耦合程度。迁移张量定义了域速度对施加到它或另一个域的力的响应,就像帆船的帆在给定施加的风力的作用下确定其速度一样。 NSE的结果提供了对蛋白质域运动性质的见解,而传统的生物物理技术则无法理解这些见解。

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