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通过电子晶体学对膜蛋白进行结构研究。

The structural study of membrane proteins by electron crystallography.

作者信息

Fujiyoshi Y

机构信息

Department of Biophysics, Faculty of Science, Kyoto University, Japan.

出版信息

Adv Biophys. 1998;35:25-80. doi: 10.1016/s0065-227x(98)90004-1.

Abstract

A high-resolution electron cryo-microscope equipped with a top-entry specimen stage has been refined by modifying a previously described superfluid helium stage. Instruments equipped with such a cryo-stage achieve a resolution of better than 2.0 A and have proved extremely powerful in the high-resolution structure analysis of membrane proteins. Improvement of the electron microscopic system in combination with improved specimen preparation techniques allowed the structure of bR to be analyzed to a resolution of 3.0 A. The 3D structure of bR, especially the surface features, revealed the structural basis for the efficient guidance of protons to the entrance of the transmembrane channel. Based on the characteristic difference of the atomic scattering factors for electrons of ionized atoms versus neutral atoms as well as the data analysis, charged and uncharged amino acid residues could be discriminated. Thus, electron crystallography is providing us with new and exciting insights into the structure of membrane proteins because it not only enables us to determine the structure of a membrane protein, but allows us to study its interaction with the surrounding lipid molecules and to determine its ionization state.

摘要

配备顶部进入式样品台的高分辨率低温电子显微镜通过改进先前描述的超流氦台得到了优化。配备这种低温台的仪器实现了优于2.0埃的分辨率,并且在膜蛋白的高分辨率结构分析中已证明具有极其强大的功能。电子显微镜系统的改进与改进的样品制备技术相结合,使得细菌视紫红质(bR)的结构能够被分析到3.0埃的分辨率。bR的三维结构,尤其是表面特征,揭示了质子有效导向跨膜通道入口的结构基础。基于离子化原子与中性原子的电子原子散射因子的特征差异以及数据分析,可以区分带电和不带电的氨基酸残基。因此,电子晶体学为我们提供了关于膜蛋白结构的全新且令人兴奋的见解,因为它不仅使我们能够确定膜蛋白的结构,还能让我们研究其与周围脂质分子的相互作用并确定其电离状态。

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