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肌肉蛋白的双功能自旋标记:通过电子顺磁共振实现精确的旋转动力学、取向和距离测定

Bifunctional Spin Labeling of Muscle Proteins: Accurate Rotational Dynamics, Orientation, and Distance by EPR.

作者信息

Thompson Andrew R, Binder Benjamin P, McCaffrey Jesse E, Svensson Bengt, Thomas David D

机构信息

Department of Biochemistry, Molecular Biology and Biophysics, University of Minnesota, Minneapolis, Minnesota, USA.

Department of Biochemistry, Molecular Biology and Biophysics, University of Minnesota, Minneapolis, Minnesota, USA.

出版信息

Methods Enzymol. 2015;564:101-23. doi: 10.1016/bs.mie.2015.06.029. Epub 2015 Aug 5.

Abstract

While EPR allows for the characterization of protein structure and function due to its exquisite sensitivity to spin label dynamics, orientation, and distance, these measurements are often limited in sensitivity due to the use of labels that are attached via flexible monofunctional bonds, incurring additional disorder and nanosecond dynamics. In this chapter, we present methods for using a bifunctional spin label (BSL) to measure muscle protein structure and dynamics. We demonstrate that bifunctional attachment eliminates nanosecond internal rotation of the spin label, thereby allowing the accurate measurement of protein backbone rotational dynamics, including microsecond-to-millisecond motions by saturation transfer EPR. BSL also allows for accurate determination of helix orientation and disorder in mechanically and magnetically aligned systems, due to the label's stereospecific attachment. Similarly, labeling with a pair of BSL greatly enhances the resolution and accuracy of distance measurements measured by double electron-electron resonance (DEER). Finally, when BSL is applied to a protein with high helical content in an assembly with high orientational order (e.g., muscle fiber or membrane), two-probe DEER experiments can be combined with single-probe EPR experiments on an oriented sample in a process we call BEER, which has the potential for ab initio high-resolution structure determination.

摘要

虽然电子顺磁共振(EPR)因其对自旋标记动力学、取向和距离具有极高的灵敏度,能够对蛋白质结构和功能进行表征,但由于使用通过柔性单功能键连接的标记,这些测量的灵敏度往往受到限制,会产生额外的无序和纳秒级动力学。在本章中,我们介绍了使用双功能自旋标记(BSL)来测量肌肉蛋白质结构和动力学的方法。我们证明,双功能连接消除了自旋标记的纳秒级内旋转,从而能够通过饱和转移EPR准确测量蛋白质主链的旋转动力学,包括微秒到毫秒级的运动。由于标记的立体特异性连接,BSL还能够在机械和磁取向系统中准确测定螺旋取向和无序度。同样,用一对BSL进行标记极大地提高了通过双电子-电子共振(DEER)测量距离的分辨率和准确性。最后,当将BSL应用于具有高螺旋含量且取向高度有序的组装体(如肌肉纤维或膜)中的蛋白质时,双探针DEER实验可以与对取向样品进行的单探针EPR实验相结合,我们将这个过程称为BEER,它具有从头进行高分辨率结构测定的潜力。

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