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首页> 外文期刊>Biochimica et biophysica acta. Biomembranes >A quantitative electrophoretic migration shift assay for analyzing the specific binding of proteins to lipid ligands in vesicles or micelles
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A quantitative electrophoretic migration shift assay for analyzing the specific binding of proteins to lipid ligands in vesicles or micelles

机译:定量电泳迁移位移分析法,用于分析蛋白质与囊泡或胶束中脂质配体的特异性结合

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摘要

We present a new assay for analyzing the specific binding of proteins to lipid ligands contained within vesicles or micelles. This assay, referred to as the electrophoretic migration shift assay, was developed using a model system composed of cholera toxin and of its physiological receptor, monosialoganglioside GM1 Using polyacrylamide gel electrophoresis in non-denaturing conditions, the migration of toxin components known to interact with GM1 was retarded when GM1 was present in either lipid vesicles or micelles. This effect was specific, as the migration of proteins not interacting with GM1 was not modified. The localization of retarded proteins and of lipids on gels was further determined by autoradiography. The stoichiometry of binding between cholera toxin and GM1 was determined, giving a value of five GM1 per one pentameric assembly of cholera toxin B-subunits, in agreement with previous studies. The general applicability of this assay was further established using both streptavidin and annexin V together with specific lipid ligands. This assay is fast, simple, quantitative, and requires only microgram quantities of protein.
机译:我们提出了一种新的分析方法,用于分析蛋白质与囊泡或胶束中所含脂质配体的特异性结合。该测定方法被称为电泳迁移转移测定法,是使用由霍乱毒素及其生理受体单唾液酸神经节苷脂GM1组成的模型系统开发的,在非变性条件下使用聚丙烯酰胺凝胶电泳,已知与GM1相互作用的毒素组分的迁移当脂质囊泡或胶束中存在GM1时,血脂水平会降低。这种作用是特异的,因为未与GM1不相互作用的蛋白质迁移没有被修饰。通过放射自显影进一步确定了阻滞蛋白和脂质在凝胶上的定位。确定了霍乱毒素和GM1之间结合的化学计量,与以前的研究一致,每一个霍乱毒素B亚基的五聚体组装得到5个GM1。同时使用链霉亲和素和膜联蛋白V以及特定的脂质配体,进一步确立了该测定法的通用性。该测定是快速,简单,定量的,并且仅需要微克量的蛋白质。

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