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Rapid screening of antibody–antigen binding using dynamic light scattering (DLS) and gold nanoparticles

机译:使用动态光散射(DLS)和金纳米颗粒快速筛选抗体-抗原结合

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A rapid one-step screening method to evaluate the specificity of antibodya€“antigen binding was developed using antibody-conjugated gold nanoparticles (Aba€“AuNPs) and dynamic light scattering (DLS). Influenza A virus was used as a model antigen to develop this platform and antigen-specific antibodies were attached to the surface of AuNPs. Introduction of virus to the nanoparticle solution resulted in aggregation of the AuNP probes provided that the antibody had an affinity for the virus. A fundamental concern of the work was to ensure aggregates only formed in the presence of the antigen. Therefore, optimal conditions for synthesizing and maintaining the stability of the Aba€“AuNP conjugates were investigated by varying pH and antibody concentration, and a protocol for preparing stable Aba€“AuNP conjugates is presented. Thereafter the AuNP probes were exploited in a DLS assay to screen the binding specificity of four antibodies to two different isolates of influenza virus (subtype H1N1). The DLS data for antibody binding were in concordance with the results obtained with a conventional ELISA, thereby validating the DLS platform. Importantly, the DLS assay was completed in 30 minutes relative to 24 hours via ELISA.
机译:使用抗体偶联的金纳米颗粒(AbaAuNPs)和动态光散射(DLS),开发了一种评估抗体与抗原结合的特异性的快速一步筛选方法。使用甲型流感病毒作为模型抗原来开发该平台,并将抗原特异性抗体附着到AuNPs的表面。如果抗体对病毒具有亲和力,则将病毒引入纳米颗粒溶液中会导致AuNP探针聚集。这项工作的基本考虑是确保仅在抗原存在下形成聚集体。因此,通过改变pH值和抗体浓度,研究了合成和维持Aba-AuNP结合物稳定性的最佳条件,并提出了制备稳定的Aba-AuNP结合物的方案。此后,在DLS分析中利用AuNP探针筛选四种抗体与两种不同流感病毒分离株(H1N1亚型)的结合特异性。抗体结合的DLS数据与常规ELISA获得的结果一致,从而验证了DLS平台。重要的是,通过ELISA,DLS分析在30分钟内完成,相对于24小时完成。

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