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Competition between bound and free peptides in an ELISA-based procedure that assays peptides derived from protein digests

机译:在基于ELISA的方法中结合肽和游离肽之间的竞争,该方法可分析源自蛋白质消化物的肽

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Background We describe an ELISA-based method that can be used to identify and quantitate proteins in biological samples. In this method, peptides in solution, derived from proteolytic digests of the sample, compete with substrate-attached synthetic peptides for antibodies, also in solution, generated against the chosen peptides. The peptides used for the ELISA are chosen on the basis of their being (i) products of the proteolytic (e.g. tryptic) digestion of the protein to be identified and (ii) unique to the target protein, as far as one can know from the published sequences. Results In this paper we describe the competition assay and we define the optimal conditions for the most effective assay. We have performed an analysis of the kinetics of interaction between the four components of the assay: the plastic substratum to which the peptide is bound, the bound peptide itself, the competing added peptide, and the antibody that is specific for the peptide and we compare the results of theoretical simulations to the actual data in some model systems. Conclusion The data suggest that the peptides bind to the plastic substratum in more than one conformation and that, once bound, the peptide displays different affinities for the antibody, depending on how it has bound to the plate
机译:背景我们描述了一种基于ELISA的方法,可用于鉴定和定量生物样品中的蛋白质。在这种方法中,源自样品蛋白水解消化液的溶液中的肽与附着于底物的合成肽争夺针对所选肽的溶液中的抗体。根据以下条件选择用于ELISA的肽段:(i)待鉴定蛋白的蛋白水解(例如胰蛋白酶)消化产物和(ii)靶蛋白特有的蛋白,据他们所知已发布的序列。结果在本文中,我们描述了竞争测定法,并定义了最有效测定法的最佳条件。我们对分析的四个组成部分之间的相互作用动力学进行了分析:与肽结合的塑料基质,与之结合的肽本身,竞争性添加的肽以及对该肽具有特异性的抗体,我们进行了比较在某些模型系统中对实际数据进行理论模拟的结果。结论数据表明,该肽以一种以上的构象与塑料基质结合,一旦结合,该肽对抗体表现出不同的亲和力,具体取决于其与板的结合方式

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