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Direct identification of protein epitopes by mass spectrometry without immobilization of antibody and isolation of antibody-peptide complexes

机译:通过质谱直接鉴定蛋白质表位,而无需固定抗体和分离抗体-肽复合物

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摘要

A rapid new approach is described that combines the selectivity and sensitivity of immunoaffinity and mass spectrometric based techniques for mapping protein epitopes. The approach alleviates the need to immobilize antibody, extract the antibody-peptide complex, and dissociate bound peptide, which are requirements of other methods. It avoids problems associated with limited proteolysis of an antigen-antibody complex particularly in the vicinity of the binding domain which can hinder identification of the epitope. Epitopic peptides are identified from a direct comparison of the matrix-assisted laser desorption ionization mass spectra of the antibody reaction mixture and an unreacted control. Samples are prepared for mass spectrometric analysis by heat-assisted and electrospray deposition to afford reproducible spectra that enable epitopic peptides to be identified in complex mixtures analyzed at the femtomole level. Indirect evidence is presented to suggest that the antibody-peptide complex is resilient to both sample deposition and the ionization event. The utility and sensitivity of the approach are illustrated for the lysozyme model. IgG-binding domains of human lysozyme are identified, and one epitope is refined to six residues that comprise part of an extended beta-loop region. [References: 33]
机译:描述了一种快速的新方法,该方法结合了免疫亲和和基于质谱的技术对蛋白质表位作图的选择性和敏感性。该方法减轻了固定抗体,提取抗体-肽复合物以及解离结合的肽的需要,这是其他方法的要求。它避免了与抗原-抗体复合物有限的蛋白水解有关的问题,特别是在结合结构域附近,这可能会阻碍表位的鉴定。从抗体反应混合物和未反应对照的基质辅助激光解吸电离质谱的直接比较中鉴定出表位肽。通过热辅助和电喷雾沉积制备样品以进行质谱分析,以提供可重现的光谱,该光谱使表位肽能够在以飞m水平分析的复杂混合物中得以鉴定。间接证据表明抗体-肽复合物对样品沉积和电离事件均具有弹性。说明了该方法的实用性和敏感性,适用于溶菌酶模型。鉴定了人溶菌酶的IgG结合结构域,并将一个表位精制为六个残基,这些残基包含一部分扩展的β环区域。 [参考:33]

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