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基于异质过渡金属的荧光偏振(HTFP)测定法用于探测蛋白质相互作用。

Heterogeneous transition metal-based fluorescence polarization (HTFP) assay for probing protein interactions.

机构信息

Institute for Organic Chemistry, University of Regensburg, Regensburg, Germany.

出版信息

Biotechniques. 2009 Oct;47(4):837-44. doi: 10.2144/000113223.

Abstract

Analyses of protein interactions are fundamental for the investigation of molecular mechanisms responsible for cellular processes and diseases, as well as for drug discovery in the pharmaceutical industry. The present study details the development of a fluorescence polarization assay using melanoma inhibitory activity (MIA) protein-binding compounds and studies of the binding properties of this protein. Since they are dependent on the the lifetime of the fluorescent label, currently available fluorescence polarization assays can only determine interactions with either high- or low-molecular weight interaction partners. Our new approach eliminates this limitation by immobilizing a known binding partner of MIA protein to a well plate and by labeling the target protein using luminescent transition metal labels such as Ru(bpy)3 for binding studies with both high- and low-molecular weight interaction partners. Due to the use of a functionalized surface, we termed our concept heterogeneous transition metal-based fluorescence polarization (HTFP) assay. The assay's independence from the molecular weight of potential binding partners should make the technique amenable to investigations on subjects as diverse as multimerization, interactions with pharmacophores, or binding affinity determination.

摘要

蛋白质相互作用分析对于研究细胞过程和疾病的分子机制以及药物发现都至关重要。本研究详细介绍了一种使用黑色素瘤抑制活性(MIA)蛋白结合化合物的荧光偏振测定法的开发,并研究了该蛋白的结合特性。由于它们依赖于荧光标记的寿命,目前可用的荧光偏振测定法只能确定与高分子量或低分子量相互作用伙伴的相互作用。我们的新方法通过将 MIA 蛋白的已知结合伙伴固定在微孔板上来消除这种限制,并使用发光过渡金属标记物(如 Ru(bpy)3)标记靶蛋白,以与高分子量和低分子量相互作用伙伴进行结合研究。由于使用了功能化表面,我们将我们的概念称为异质过渡金属基荧光偏振(HTFP)测定法。该测定法不依赖于潜在结合伙伴的分子量,这使得该技术适用于各种研究,如多聚化、与药效团的相互作用或结合亲和力的测定。

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