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Dissecting coherent vibrational spectra of small proteins into secondary structural elements by sensitivity analysis

机译:通过敏感性分析将小蛋白的相干振动光谱分解为二级结构元素

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摘要

The response of proteins to sequences of femtosecond infrared pulses provides a multidimensional view into their equilibrium distribution of structures and snapshot pictures of fast-triggered dynamical events. Analyzing these experiments requires advanced computational tools for assigning regions in the resulting multi-dimensional correlation plots to specific secondary-structure elements and their couplings. A differential sensitivity analysis technique based on a perturbation of the local (real space) Hamiltonian is developed to achieve that goal. Application to the amide I region of a small globular protein reveals regions associated with the α-helix, β-sheet, and their coupling. Comparison of signals generated in different directions shows that the double-quantum-coherence signal has a higher sensitivity to the couplings compared with the single-quantum-coherence (photon echo) technique.
机译:蛋白质对飞秒红外脉冲序列的响应提供了对其结构的均衡分布和快速触发的动态事件的快照图片的多维视图。分析这些实验需要先进的计算工具,以便将所得多维相关图中的区域分配给特定的二级结构元素及其耦合。为了实现该目标,开发了一种基于局部(真实空间)哈密顿量摄动的差分灵敏度分析技术。应用于小球状蛋白的酰胺I区可揭示与α-螺旋,β-折叠及其偶联相关的区域。比较不同方向产生的信号表明,与单量子相干(光子回波)技术相比,双量子相干信号对耦合具有更高的灵敏度。

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