用一种合成荧光氨基酸探究蛋白质静电学

Probing protein electrostatics with a synthetic fluorescent amino acid.

作者信息

Cohen Bruce E, McAnaney Tim B, Park Eun Sun, Jan Yuh Nung, Boxer Steven G, Jan Lily Yeh

机构信息

Howard Hughes Medical Institute and Departments of Physiology and Biochemistry, University of California San Francisco, San Francisco, CA 94143, USA.

出版信息

Science. 2002 May 31;296(5573):1700-3. doi: 10.1126/science.1069346.

DOI:10.1126/science.1069346

PMID:12040199

Abstract

Electrostatics affect virtually all aspects of protein structure and activity and are particularly important in proteins whose primary function is to stabilize charge. Here we introduce a fluorescent amino acid, Aladan, which can probe the electrostatic character of a protein at multiple sites. Aladan is exceptionally sensitive to the polarity of its surroundings and can be incorporated site-selectively at buried and exposed sites, in both soluble and membrane proteins. Steady-state and time-resolved fluorescence measurements of Aladan residues at different buried and exposed sites in the B1 domain of protein G suggest that its interior is polar and heterogeneous.

摘要

静电作用几乎影响蛋白质结构和活性的各个方面，在主要功能是稳定电荷的蛋白质中尤为重要。在此，我们引入了一种荧光氨基酸阿拉丹（Aladan），它可以在多个位点探测蛋白质的静电特性。阿拉丹对其周围环境的极性异常敏感，并且可以位点选择性地掺入可溶性和膜蛋白的埋藏位点和暴露位点。对蛋白质G的B1结构域中不同埋藏和暴露位点的阿拉丹残基进行稳态和时间分辨荧光测量表明，其内部是极性且异质的。

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用一种合成荧光氨基酸探究蛋白质静电学

Probing protein electrostatics with a synthetic fluorescent amino acid.

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