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Homogeneous Fluorescence-Based Immunoassay Detects Antigens Within 90 Seconds

机译:均相荧光免疫分析法可在90秒内检测出抗原

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Homogeneous immunoassays are prevalent tools for the detection of antigens. The major advantage over heterogeneous immunoassays is the absence of numerous incubation and washing steps, reducing the assay time and allowing rapid on-site detection of antigens (e.g., toxins and pollutants). The simple experimental setup of a homogeneous immunoassay also allows a robust analysis even when performed by non-laboratory-trained personnel. Here we present a homogeneous immunoassay for the rapid determination of antigens. As a proof of concept, a phosphorylation-specific anti-human tau monoclonal antibody was labeled with an acceptor and the corresponding peptide probe with a donor fluorophore. The analyte sample is spiked with a fixed amount of donor peptide before acceptor-labeled antibody is added leading to a donor fluorescence quenching. Thus the intensity of the fluorescence signal of the donor peptide probe depends on the concentration of the target antigen. The sequence of the donor peptide was optimized to lower its affinity to the antibody giving a higher response for the analyte antigen compared to the native epitope. This allowed a semiquantitative analysis of the antigen within only 90 s.
机译:均相免疫测定是检测抗原的普遍工具。相对于异源免疫测定法的主要优点是无需进行大量的孵育和洗涤步骤,从而缩短了测定时间并可以快速现场检测抗原(例如毒素和污染物)。均质免疫测定的简单实验设置也允许进行可靠的分析,即使由未经实验室培训的人员进行也是如此。在这里,我们提出了一种用于快速测定抗原的均相免疫测定法。作为概念的证明,磷酸化特异性抗人tau单克隆抗体用受体标记,相应的肽探针用供体荧光团标记。在添加受体标记的抗体导致供体荧光猝灭之前,向分析物样品添加固定量的供体肽。因此,供体肽探针的荧光信号的强度取决于靶抗原的浓度。优化了供体肽的序列,以降低其对抗体的亲和力,与天然表位相比,对分析物抗原的响应更高。这样可以在90 s内对抗原进行半定量分析。

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