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用于膜结合蛋白在线表征和靶向亲和分离的固定化膜基亲和柱的开发。

Development of immobilized membrane-based affinity columns for use in the online characterization of membrane bound proteins and for targeted affinity isolations.

作者信息

Moaddel Ruin, Wainer Irving W

机构信息

Gerontology Research Center, National Institute on Aging, National Institutes of Health, 5600 Nathan Shock Drive, Baltimore, MD 21224-6825, USA.

出版信息

Anal Chim Acta. 2006 Mar 30;564(1):97-105. doi: 10.1016/j.aca.2005.09.020. Epub 2005 Oct 19.

DOI:10.1016/j.aca.2005.09.020
PMID:17723367
Abstract

Membranes obtained from cell lines that express or do not express a target membrane bound protein have been immobilized on a silica-based liquid chromatographic support or on the surface of an activated glass capillary. The resulting chromatographic columns have been placed in liquid chromatographic systems and used to characterize the target proteins and to identify small molecules that bind to the target. Membranes containing ligand gated ion channels, G-protein coupled receptors and drug transporters have been prepared and characterized. If a marker ligand has been identified for the target protein, frontal or zonal displacement chromatographic techniques can be used to determine binding affinities (K(d) values) and non-linear chromatography can be used to assess the association (k(on)) and dissociation (k(off)) rate constants and the thermodynamics of the binding process. Membrane-based affinity columns have been created using membranes from a cell line that does not express the target protein (control) and the same cell line that expresses the target protein (experimental) after genomic transfection. The resulting columns can be placed in a parallel chromatography system and the differential retention between the control and experimental columns can be used to identify small molecules and protein that bind to the target protein. These applications will be illustrated using columns created using cellular membranes containing nicotinic acetylcholine receptors and the drug transporter P-glycoprotein.

摘要

从表达或不表达目标膜结合蛋白的细胞系获得的膜已固定在基于硅胶的液相色谱支持物上或活化玻璃毛细管的表面。所得的色谱柱已放置在液相色谱系统中,用于表征目标蛋白并鉴定与目标结合的小分子。已制备并表征了含有配体门控离子通道、G蛋白偶联受体和药物转运蛋白的膜。如果已鉴定出目标蛋白的标记配体,则可使用前沿或区域置换色谱技术来确定结合亲和力(K(d)值),并且可使用非线性色谱来评估缔合(k(on))和解离(k(off))速率常数以及结合过程的热力学。在基因组转染后,已使用来自不表达目标蛋白的细胞系(对照)和表达目标蛋白的同一细胞系(实验)的膜创建了基于膜的亲和柱。所得的柱可放置在平行色谱系统中,并且对照柱和实验柱之间的差异保留可用于鉴定与目标蛋白结合的小分子和蛋白质。将使用含有烟碱型乙酰胆碱受体和药物转运蛋白P-糖蛋白的细胞膜创建的柱来说明这些应用。

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