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DNA 定向固定与免疫聚合酶链反应相结合:借助自组装 DNA-蛋白质缀合物进行超灵敏抗原检测。

Combination of DNA-directed immobilization and immuno-PCR: very sensitive antigen detection by means of self-assembled DNA-protein conjugates.

作者信息

Niemeyer Christof M, Wacker Ron, Adler Michael

机构信息

Universität Dortmund, Fachbereich Chemie, Biologisch-Chemische Mikrostrukturtechnik, Otto-Hahn-Strasse 6, D-44227 Dortmund, Germany.

出版信息

Nucleic Acids Res. 2003 Aug 15;31(16):e90. doi: 10.1093/nar/gng090.

DOI:10.1093/nar/gng090
PMID:12907742
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC169982/
Abstract

An assay for very sensitive antigen detection is described which takes advantage of the self- assembly capabilities of semi-synthetic conjugates of DNA and proteins. The general scheme of this assay is similar to a two-sided (sandwich) enzyme-linked immunoassay (ELISA); however, covalent single-stranded DNA-streptavidin (STV) conjugates, capable of hybridizing to complementary surface-bound DNA oligomers, are utilized for the effective immobilization of either capture antibodies or antigens, rather than the chemi- or physisorption usually applied in ELISA. Immuno-PCR (IPCR) is employed as a method for signal generation, utilizing oligomeric reagents obtained by self-assembly of STV, biotinylated DNA and antibodies. In three different model systems, detecting human IgG, rabbit IgG or carcinoembryonic antigen, this combination allowed one to increase the sensitivity of the analogous ELISA approximately 1000-fold. For example, <0.1 amol/ micro l (15 pg/ml) of rabbit IgG was detectable. The immunoassay can be carried out in a single step by tagging the analyte with both reagents for capture and read-out simultaneously, thereby significantly reducing handling time and costs of analysis. Moreover, as the spatial selectivity of target immobilization is determined by the specificity of DNA base pairing, the assay is particularly suited for miniaturized microfluidics and lab-on-a-chip devices.

摘要

本文描述了一种用于超灵敏抗原检测的分析方法,该方法利用了DNA与蛋白质的半合成缀合物的自组装能力。该分析方法的总体方案类似于双面(夹心)酶联免疫吸附测定法(ELISA);然而,能够与互补的表面结合DNA寡聚物杂交的共价单链DNA-链霉亲和素(STV)缀合物,被用于有效固定捕获抗体或抗原,而不是ELISA中通常采用的化学吸附或物理吸附。免疫聚合酶链反应(IPCR)被用作信号产生的方法,利用通过STV、生物素化DNA和抗体自组装获得的寡聚试剂。在检测人IgG、兔IgG或癌胚抗原的三种不同模型系统中,这种组合使类似ELISA的灵敏度提高了约1000倍。例如,可检测到<0.1 amol/μl(15 pg/ml)的兔IgG。该免疫测定法可以通过同时用捕获和读出试剂标记分析物在一步中进行,从而显著减少处理时间和分析成本。此外,由于靶标固定的空间选择性由DNA碱基配对的特异性决定,该测定法特别适用于小型化的微流控和芯片实验室设备。

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