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使用定点荧光标记和双硫腙衍生物(2-吡啶基)二硫代双硫腙进行高通量蛋白质结构分析。

High-throughput protein structural analysis using site-directed fluorescence labeling and the bimane derivative (2-pyridyl)dithiobimane.

作者信息

Mansoor Steven E, Farrens David L

机构信息

Department of Biochemistry and Molecular Biology, Oregon Health and Science University, 3181 SW Sam Jackson Park Road, Portland, Oregon 97239-3098, USA.

出版信息

Biochemistry. 2004 Jul 27;43(29):9426-38. doi: 10.1021/bi036259m.

Abstract

We present a site-directed fluorescence labeling (SDFL) study of 25 different T4 lysozyme protein samples labeled with the thiol-cleavable fluorophore, (2-pyridyl)dithiobimane (PDT-Bimane). Our results demonstrate PDT-Bimane can be used in cysteine-scanning studies to detect protein secondary structure, and to map proximity between sites in proteins by monitoring tryptophan quenching of bimane fluorescence. In addition, the reducible nature of PDT-Bimane can be exploited to resolve problems often faced in SDFL studies: ensuring specific labeling of cysteine residues, determining the extent of free label contamination, and accurately determining labeling efficiency even at low concentrations. The ability to cleave PDT-Bimane off the protein enables rapid determination of these parameters, and positions it as an ideal fluorophore for automated, high-throughput structural studies of protein folding, the detection of protein-protein interactions, and the monitoring of real-time conformational changes.

摘要

我们展示了一项针对25种不同的T4溶菌酶蛋白样品的定点荧光标记(SDFL)研究,这些样品用可被硫醇裂解的荧光团(2-吡啶基)二硫代双马来酰亚胺(PDT-双马来酰亚胺)进行了标记。我们的结果表明,PDT-双马来酰亚胺可用于半胱氨酸扫描研究,以检测蛋白质二级结构,并通过监测双马来酰亚胺荧光的色氨酸猝灭来绘制蛋白质中位点之间的距离。此外,PDT-双马来酰亚胺的可还原性质可用于解决SDFL研究中经常遇到的问题:确保半胱氨酸残基的特异性标记、确定游离标记污染的程度以及即使在低浓度下也能准确确定标记效率。将PDT-双马来酰亚胺从蛋白质上裂解下来的能力能够快速确定这些参数,并使其成为蛋白质折叠的自动化、高通量结构研究、蛋白质-蛋白质相互作用检测以及实时构象变化监测的理想荧光团。

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