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膜蛋白的定点13C固态核磁共振研究:以[1-13C]氨基酸残基标记的细菌视紫红质为例揭示构象和动力学的策略与目标

Site-directed 13C solid-state NMR studies on membrane proteins: strategy and goals toward revealing conformation and dynamics as illustrated for bacteriorhodopsin labeled with [1-13C]amino acid residues.

作者信息

Saitô Hazime, Mikami Jun, Yamaguchi Satoru, Tanio Michikazu, Kira Atushi, Arakawa Tadashi, Yamamoto Kazutoshi, Tuzi Satoru

机构信息

Department of Life Science, Graduate School of Science, Himeji Institute of Technology, Harima Science Garden City, Kamigori, Hyogo 678-1297, Japan.

出版信息

Magn Reson Chem. 2004 Feb;42(2):218-30. doi: 10.1002/mrc.1325.

Abstract

We have so far demonstrated that well-resolved and site-specifically assigned (13)C peaks as recorded by site-directed NMR study on (13)C-labeled membrane proteins can serve as a convenient probe to reveal their local conformation and dynamics. We attempted here to clarify the extent to which (13)C NMR spectra of (13)C-labeled fully hydrated bacteriorhodopsin (bR) as a typical membrane protein are visible or well resolved in the presence of inherent fluctuation motions with frequency of 10(2)-10(8) Hz, especially at the membrane surfaces. Accordingly, we estimated the relative proportion of (13)C NMR signals from the surface areas with and without peak suppression by the accelerated transverse relaxation effect by surface-bound Mn(2+) ions, which could be effective for residues within 8.7 angstroms of the membrane surface. It turned out that the experimental findings are consistent with the predicted amount of amino acid residues under consideration located within 8.7 angstroms of the surface for [1-(13)C]Val- and Ile-labeled bR and also [3-(13)C]Ala-bR. In contrast, (13)C NMR peaks from such surfaces area are almost completely or partially suppressed for [1-(13)C]Gly-, Ala-, Leu-, Phe- and Trp-labeled bR, as a result of plausible interference of the fluctuation frequency with frequency of magic angle spinning (10(4) Hz). We further assigned several (13)C NMR signals of [1-(13)C] Val-, Trp- and Ile-labeled bR on the basis of a variety of site-directed mutants with reference to those of the wild type. Further, we recorded the (13)C NMR of bR in lipid bilayers to search for the optimal conditions to be able to obtain signals with the highest peak intensities and spectral resolution. Backbone dynamics turn out to be essential for recording (13)C NMR spectra so as to escape from motional frequencies of the order of 10(4)-10(5) Hz, either in the direction of accelerated fluctuation or slowed motions in the direction of forming the 2D array.

摘要

到目前为止,我们已经证明,通过对13C标记的膜蛋白进行定点核磁共振研究记录的分辨率良好且位点特异性归属的13C峰,可以作为揭示其局部构象和动力学的便捷探针。我们在此试图阐明,作为典型膜蛋白的13C标记的完全水合细菌视紫红质(bR)的13C核磁共振谱,在存在频率为102-108Hz的固有波动运动的情况下,尤其是在膜表面,在何种程度上是可见的或分辨率良好的。因此,我们估计了来自有和没有表面结合的Mn2+离子加速横向弛豫效应导致的峰抑制的表面积的13C核磁共振信号的相对比例,这对膜表面8.7埃内的残基可能是有效的。结果表明,实验结果与预测的[1-(13)C]Val-和Ile-标记的bR以及[3-(13)C]Ala-bR表面8.7埃内的氨基酸残基数量一致。相比之下,对于[1-(13)C]Gly-、Ala-、Leu-、Phe-和Trp-标记的bR,由于波动频率与魔角旋转频率(104Hz)的合理干扰,来自此类表面积的13C核磁共振峰几乎完全或部分被抑制。我们还基于各种定点突变体,并参考野生型的突变体,对[1-(13)C]Val-、Trp-和Ile-标记的bR的几个13C核磁共振信号进行了归属。此外,我们记录了脂质双层中bR的13C核磁共振谱,以寻找能够获得具有最高峰强度和光谱分辨率的信号的最佳条件。结果表明,主链动力学对于记录13C核磁共振谱至关重要,以便在加速波动方向或形成二维阵列方向的慢运动方向上避开104-105Hz量级的运动频率。

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