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Coherence Spectroscopy Investigations of the Low-Frequency Vibrations of Heme: Effects of Protein-Specific Perturbations

机译:血红素低频振动的相干光谱研究:蛋白质特有摄动的影响

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摘要

Femtosecond coherence spectroscopy is used to probe the low-frequency (20–200 cm−1) vibrational modes of heme proteins in solution. Horseradish peroxidase (HRP), myoglobin (Mb), and Campylobacter jejuni globin (Cgb) are compared and significant differences in the coherence spectra are revealed. It is concluded that hydrogen bonding and ligand charge do not strongly affect the low-frequency coherence spectra and that protein-specific deformations of the heme group lower its symmetry and control the relative spectral intensities. Such deformations potentially provide a means for proteins to tune heme reaction coordinates, so that they can perform a broad array of specific functions. Native HRP displays complex spectral behavior above ~50 cm−1 and very weak activity below ~50 cm−1. Binding of the substrate analog, benzhydroxamic acid, leads to distinct changes in the coherence and Raman spectra of HRP that are consistent with the stabilization of a heme water ligand. The CN derivatives of the three proteins are studied to make comparisons under conditions of uniform heme coordination and spin-state. MbCN is dominated by a doming mode near 40 cm−1, while HRPCN displays a strong oscillation at higher frequency (96 cm−1) that can be correlated with the saddling distortion observed in the X-ray structure. In contrast, CgbCN displays low-frequency coherence spectra that contain strong modes near 30 and 80 cm−1, probably associated with a combination of heme doming and ruffling. HRPNO displays a strong doming mode near 40 cm−1 that is activated by photolysis. The damping of the coherent motions is significantly reduced when the heme is shielded from solvent fluctuations by the protein material and reduced still further when T ≲ 50 K, as pure dephasing processes due to the protein–solvent phonon bath are frozen out.
机译:飞秒相干光谱用于探测溶液中血红素蛋白的低频(20–200 cm -1 )振动模式。比较了辣根过氧化物酶(HRP),肌红蛋白(Mb)和空肠弯曲杆菌球蛋白(Cgb),并揭示了相干光谱的显着差异。结论是氢键和配体电荷不会强烈影响低频相干光谱,血红素基团的蛋白质特异性变形降低了其对称性并控制了相对光谱强度。这样的变形潜在地为蛋白质提供了调节血红素反应坐标的手段,从而它们可以执行各种各样的特定功能。天然HRP在〜50 cm -1 以上显示复杂的光谱行为,而在〜50 cm -1 以下显示非常弱的活性。底物类似物苯氧肟酸的结合导致HRP的相干性和拉曼光谱发生明显变化,这与血红素水配体的稳定化相一致。研究了这三种蛋白质的CN衍生物,以在血红素均匀配位和自旋态条件下进行比较。 MbCN由40 cm -1 附近的隆起模式主导,而HRPCN在较高的频率(96 cm -1 )上显示出强烈的振荡,这可能与鞍形失真相关在X射线结构中观察到。相反,CgbCN显示的低频相干光谱在30和80 cm -1 附近包含强模式,可能与血红素隆起和波纹相关。 HRPNO在40 cm -1 附近显示出很强的穹顶模式,该模式被光解激活。当血红素被蛋白质材料屏蔽而不受溶剂波动影响时,相干运动的阻尼将显着降低,而当T≲50 K时,由于蛋白质-溶剂声子浴导致的纯相移过程被冻结,相干运动的阻尼将进一步降低。

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