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Immunoassays with Direct Mass Spectrometric Detection

机译:直接质谱检测的免疫分析

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摘要

A rapid, specific, and sensitive method for the detection of protein-protein interactions is of crucial importance for drug discovery and clinical diagnostics. Mass spectrometry plays a major role in the analysis of proteins, but its application to the routine analysis of protein complexes has been lagging behind. A new strategy for high-throughput analysis of protein interactions is presented here. We demonstrate application to immunochemical questions such as epitope mapping, kinetic studies, and sandwich assays. The methodology is based on a direct mass spectrometric readout for antigen-antibody complexes in the 150-400 kDa range. This has become possible using a novel detector technology and chemical cross-linking to stabilize complexes for analysis by MALDI MS. We demonstrate high detection sensitivity (femtomole quantities of antigen), high specificity (specific detection of antigen directly in serum), high accuracy, and high speed (minutes per assay), surpassing conventional analytical methods by more than 2 orders of magnitude.
机译:快速,特异性和灵敏的蛋白质-蛋白质相互作用检测方法对于药物发现和临床诊断至关重要。质谱法在蛋白质分析中起主要作用,但在蛋白质复合物常规分析中的应用一直滞后。本文介绍了一种高通量分析蛋白质相互作用的新策略。我们证明了对免疫化学问题的应用,例如表位作图,动力学研究和夹心测定。该方法基于150-400 kDa范围内抗原-抗体复合物的直接质谱读数。使用新型检测器技术和化学交联来稳定复合物以通过MALDI MS进行分析,这已成为可能。我们证明了高检测灵敏度(抗原中的飞沫数量),高特异性(直接在血清中进行抗原的特异性检测),高精度和高速度(每个测定分钟),比传统的分析方法高出两个数量级。

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