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将(19)F-氨基酸位点特异性掺入蛋白质中作为用于表征蛋白质结构和反应性的核磁共振探针。

Site-specific incorporation of a (19)F-amino acid into proteins as an NMR probe for characterizing protein structure and reactivity.

作者信息

Jackson Jennifer C, Hammill Jared T, Mehl Ryan A

机构信息

Department of Chemistry, Franklin and Marshall College, P.O. Box 3003, Lancaster, Pennsylvania 17604, USA.

出版信息

J Am Chem Soc. 2007 Feb 7;129(5):1160-6. doi: 10.1021/ja064661t.

Abstract

19F NMR is a powerful tool for monitoring protein conformational changes and interactions; however, the inability to site-specifically introduce fluorine labels into proteins of biological interest severely limits its applicability. Using methods for genetically directing incorporation of unnatural amino acids, we have inserted trifluoromethyl-l-phenylalanine (tfm-Phe) into proteins in vivo at TAG nonsense codons with high translational efficiency and fidelity. The binding of substrates, inhibitors, and cofactors, as well as reactions in enzymes, were studied by selective introduction of tfm-Phe and subsequent monitoring of the 19F NMR chemical shifts. Subtle protein conformational changes were detected near the active site and at long distances (25 Angstrom). 19F signal sensitivity and resolution was also sufficient to differentiate protein environments in vivo. Since there has been interest in using 19F-labeled proteins in solid-state membrane protein studies, folding studies, and in vivo studies, this general method for genetically incorporating a 19F-label into proteins of any size in Escherichia coli should have broad application beyond that of monitoring protein conformational changes.

摘要

19F核磁共振是监测蛋白质构象变化和相互作用的有力工具;然而,无法将氟标签位点特异性地引入具有生物学意义的蛋白质中,这严重限制了其适用性。利用基因指导非天然氨基酸掺入的方法,我们已在体内将三氟甲基-L-苯丙氨酸(tfm-Phe)插入到TAG无义密码子的蛋白质中,具有较高的翻译效率和保真度。通过选择性引入tfm-Phe并随后监测19F核磁共振化学位移,研究了底物、抑制剂和辅因子的结合以及酶中的反应。在活性位点附近和远距离(25埃)处检测到了细微的蛋白质构象变化。19F信号的灵敏度和分辨率也足以区分体内的蛋白质环境。由于人们对在固态膜蛋白研究、折叠研究和体内研究中使用19F标记的蛋白质感兴趣,这种在大肠杆菌中基因掺入19F标签到任何大小蛋白质中的通用方法,其应用范围应比监测蛋白质构象变化更为广泛。

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