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酶活性位点处的电场:实验与理论的直接比较

Electric fields at the active site of an enzyme: direct comparison of experiment with theory.

作者信息

Suydam Ian T, Snow Christopher D, Pande Vijay S, Boxer Steven G

机构信息

Department of Chemistry, Stanford University, Stanford, CA 94305-5080, USA.

出版信息

Science. 2006 Jul 14;313(5784):200-4. doi: 10.1126/science.1127159.

Abstract

The electric fields produced in folded proteins influence nearly every aspect of protein function. We present a vibrational spectroscopy technique that measures changes in electric field at a specific site of a protein as shifts in frequency (Stark shifts) of a calibrated nitrile vibration. A nitrile-containing inhibitor is used to deliver a unique probe vibration to the active site of human aldose reductase, and the response of the nitrile stretch frequency is measured for a series of mutations in the enzyme active site. These shifts yield quantitative information on electric fields that can be directly compared with electrostatics calculations. We show that extensive molecular dynamics simulations and ensemble averaging are required to reproduce the observed changes in field.

摘要

折叠蛋白质中产生的电场几乎影响蛋白质功能的方方面面。我们提出了一种振动光谱技术,该技术通过校准腈振动的频率变化(斯塔克位移)来测量蛋白质特定位点处电场的变化。一种含腈抑制剂被用于将独特的探针振动传递到人醛糖还原酶的活性位点,并针对该酶活性位点的一系列突变测量腈伸缩频率的响应。这些位移产生了关于电场的定量信息,可直接与静电计算结果进行比较。我们表明,需要进行广泛的分子动力学模拟和系综平均来重现观察到的场变化。

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