噬菌体抗免疫复合物分析:小分子非竞争性免疫检测的通用策略。
Phage anti-immune complex assay: general strategy for noncompetitive immunodetection of small molecules.
作者信息
González-Techera A, Vanrell L, Last J A, Hammock B D, González-Sapienza G
机构信息
Cátedra de Inmunología, Facultad de Química, Instituto de Higiene, UDELAR, Montevideo, Uruguay 11600.
出版信息
Anal Chem. 2007 Oct 15;79(20):7799-806. doi: 10.1021/ac071323h. Epub 2007 Sep 11.
Abstract
Due to their size, small molecules cannot be simultaneously bound by two antibodies, precluding their detection by noncompetitive two-site immunoassays, which are superior to competitive ones in terms of sensitivity, kinetics, and working range. This has prompted the development of anti-immune complex antibodies, but these are difficult to produce, and often exhibit high cross-reactivity with the unliganded primary antibody. This work demonstrates that anti-immune complex antibodies can be substituted by phage particles isolated from phage display peptide libraries. Phages bearing specific small peptide loops allowed to focus the recognition to changes in the binding area of the immune complex. The concept was tested using environmental and drug analytes; with improved sensitivity and ready adaptation into on-site formats. Peptides specific for different immune complexes can be isolated from different peptide libraries in a simple and systematic fashion allowing the rapid development of noncompetitive assays for small molecules.
摘要
由于小分子的尺寸,它们不能同时被两种抗体结合,这使得它们无法通过非竞争性双位点免疫测定法进行检测,而非竞争性双位点免疫测定法在灵敏度、动力学和工作范围方面优于竞争性免疫测定法。这促使了抗免疫复合物抗体的开发,但这些抗体难以生产,并且通常与未结合配体的一级抗体表现出高交叉反应性。这项工作表明,抗免疫复合物抗体可以被从噬菌体展示肽库中分离出的噬菌体颗粒所替代。带有特定小肽环的噬菌体能够将识别聚焦于免疫复合物结合区域的变化。该概念已通过环境和药物分析物进行了测试,具有更高的灵敏度并且易于适配到现场检测形式中。可以以简单且系统的方式从不同的肽库中分离出针对不同免疫复合物的肽,从而实现小分子非竞争性测定法的快速开发。
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