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Vibrational Stark Effects of Carbonyl Probes Applied to Re-interpret IR and Raman Data for Enzyme Inhibitors in Terms of Electric Fields at the Active Site

机译:羰基探针的振动斯塔克效应用于根据活性部位的电场重新解释酶抑制剂的IR和拉曼数据

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摘要

IR and Raman frequency shifts have been reported for numerous probes of enzyme transition states, leading to diverse interpretations. In the case of the model enzyme ketosteroid isomerase (KSI), we have argued that IR spectral shifts for a carbonyl probe at the active site can provide a connection between the active site electric field and the activation free energy (Fried et al. Science, >2014, 346, 1510–1514). Here we generalize this approach to a much broader set of carbonyl probes (e.g. oxoesters, thioesters, and amides), first establishing the sensitivity of each probe to an electric field using vibrational Stark spectroscopy, vibrational solvatochromism, and MD simulations, and then applying these results to re-interpret data already in the literature for enzymes such as 4-chlorobenzoyl-CoA dehalogenase and serine proteases. These results demonstrate that the vibrational Stark effect provides a general framework for estimating the electrostatic contribution to the catalytic rate and may provide a metric for the design or modification of enzymes. Opportunities and limitations of the approach are also described.
机译:已经报道了许多酶跃迁状态探针的IR和拉曼频移,导致了多种解释。在模型酶酮类固醇异构酶(KSI)的情况下,我们认为羰基探针在活性位点处的IR光谱位移可以在活性位点电场和活化自由能之间建立联系(Fried等人, > 2014 ,346,1510–1514)。在这里,我们将这种方法推广到更广泛的羰基探针组(例如,含氧酸酯,硫酯和酰胺),首先使用振动斯塔克光谱,振动溶剂化和MD模拟建立每个探针对电场的敏感性,然后应用这些方法结果重新诠释了文献中有关4-氯苯甲酰辅酶A脱卤素酶和丝氨酸蛋白酶的数据。这些结果表明,振动斯塔克效应为估计静电对催化速率的贡献提供了一般框架,并且可以为酶的设计或修饰提供度量。还介绍了该方法的机会和局限性。

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  • 年(卷),期 -1(120),36
  • 年度 -1
  • 页码 9672–9684
  • 总页数 27
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