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Construction of an antibody microarray based on agarose-coated slides.

机译:基于琼脂糖涂层载玻片的抗体微阵列的构建。

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The antibody microarray, a high-throughput multiplex immunoassay method, has become a significant tool for quantitative proteomics studies. We describe here the strategies for optimizing the condition of antibody microarray building based on agarose-coated slides. In this study, modified glass slides were robotically printed with capture antibodies against monocyte chemoattractant protein 1 (MCP-1), then dilutions of the cytokine were applied to the arrays, and the protein was detected with biotin-labeled antibody coupled with Cy3-conjugated streptavidin. Thus a protein profiling microarray based on sandwich immunoassay has been established. Various factors in the production of antibody microarrays were analyzed: the capture antibody concentrations, shelf life of the postprinting slides, blocking buffers, and reproducibility of the system. A calibration curve with a correlation coefficient of 0.9995 was established which suggested that the matrix can retain arrayed proteins in near-quantitative fashion. The results revealed high signal uniformity and reproducibility with regard to intra-array (1.3%) and the interarray (8.7%) variation at the capture antibody concentration of 125 microg/mL. Besides, the printed arrays could be stored for at least two months without any apparent change of the performance parameters.
机译:抗体微阵列是一种高通量的多重免疫分析方法,已成为定量蛋白质组学研究的重要工具。我们在此处描述了基于琼脂糖涂层载玻片优化抗体微阵列构建条件的策略。在这项研究中,用抗单核细胞趋化蛋白1(MCP-1)的捕获抗体自动印刷修饰的载玻片,然后将细胞因子稀释液应用于阵列,并用生物素标记的抗体与Cy3偶联的蛋白检测该蛋白。链霉亲和素。因此,已经建立了基于夹心免疫测定的蛋白质谱分析微阵列。分析了抗体微阵列生产中的各种因素:捕获抗体的浓度,印后载玻片的保质期,封闭缓冲液和系统的可重复性。建立了相关系数为0.9995的校准曲线,这表明基质可以以接近定量的方式保留阵列蛋白。结果显示,在捕获抗体浓度为125 microg / mL时,阵列内(1.3%)和阵列间(8.7%)变异具有很高的信号均匀性和可重复性。此外,印刷的阵列可以存储至少两个月,而性能参数没有任何明显的变化。

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