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利用非经典金属氨基酸 [Cu(II)(2,2'-联吡啶-5-基)]-丙氨酸研究蛋白质结构。

Using the Noncanonical Metallo-Amino Acid [Cu(II)(2,2'-Bipyridin-5-yl)]-alanine to Study the Structures of Proteins.

机构信息

Institute for Integrative Biology of the Cell, Department of Biochemistry, Biophysics and Structural Biology, Université Paris-Saclay, CEA, CNRS UMR 9198, CEA-Saclay, Gif-sur-Yvette F-91198, France.

Institut de Chimie Moléculaire et des Matériaux d'Orsay (ICMMO), Université Paris-Saclay, CNRS, Orsay F-91405, Cedex France.

出版信息

J Phys Chem Lett. 2023 Apr 13;14(14):3368-3375. doi: 10.1021/acs.jpclett.3c00196. Epub 2023 Mar 30.

Abstract

Genetic code expansion allows modification of the physical and chemical properties of proteins by the site-directed insertion of noncanonical amino acids. Here we exploit this technology for measuring nanometer-scale distances in proteins. (2,2'-Bipyridin-5-yl)alanine was incorporated into the green fluorescent protein (GFP) and used as an anchoring point for Cu(II) to create a spin-label. The incorporation of (2,2'-bipyridin-5-yl)alanine directly into the protein resulted in a high-affinity binding site for Cu(II) capable of outcompeting other binding positions in the protein. The resulting Cu(II)-spin label is very compact and not larger than a conventional amino acid. By using 94 GHz electron paramagnetic resonance (EPR) pulse dipolar spectroscopy we have been able to determine accurately the distance between two such spin-labels. Our measurements revealed that GFP dimers can adopt different quaternary conformations. The combination of spin-labeling using a paramagnetic nonconventional amino acid with high-frequency EPR techniques resulted in a sensitive method for studying the structures of proteins.

摘要

遗传密码扩展允许通过定点插入非规范氨基酸来修饰蛋白质的物理和化学性质。在这里,我们利用这项技术来测量蛋白质中的纳米级距离。(2,2'-联吡啶-5-基)丙氨酸被掺入绿色荧光蛋白(GFP)中,并用作 Cu(II)的锚固点以形成自旋标记。(2,2'-联吡啶-5-基)丙氨酸直接掺入蛋白质中会产生一个高亲和力的 Cu(II)结合位点,能够与蛋白质中的其他结合位置竞争。所得的 Cu(II)-自旋标记非常紧凑,不大于常规氨基酸。通过使用 94 GHz 电子顺磁共振(EPR)脉冲偶极子光谱法,我们能够准确地确定两个这样的自旋标记之间的距离。我们的测量结果表明,GFP 二聚体可以采用不同的四级构象。使用顺磁非规范氨基酸和高频 EPR 技术进行自旋标记的组合产生了一种用于研究蛋白质结构的灵敏方法。

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