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An Indirect Immunoassay for Detecting Antigen Based on Fluorescence Resonance Energy Transfer

机译:基于荧光共振能量转移的间接免疫检测抗原

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摘要

An indirect immunoassay for detecting antigen was developed. It was based on fluorescence resonance energy transfer (FRET) and quenching of gold nanoparticles. Bovine serum albumin (BSA) was chosen as model antigen. Fluorescein isothiocyanate (FITC) was attached to anti-BSA antibody (anti-BSA–FITC) as FRET donor, while BSA was conjugated to gold nanoparticles (GNPs–BSA) as FRET acceptor. The formation of anti-BSA–BSA immunocomplex resulted in the FRET between anti-BSA–FITC and GNPs–BSA. Thus, the fluorescence of FRET donor was quenched, and the decreasing fluorescence intensity responded linearly to the concentration of acceptor within the linear range. The concentration of BSA we obtained according to the stoichiometric ratio between BSA and GNPs. Following this approach, we were able to specifically detect BSA. The detection limit for BSA was 0.5 nM and the linear range of the assay was 2.9 - 43.5 nM. It had been successfully applied to specific detection of BSA in serum samples.
机译:开发了用于检测抗原的间接免疫测定法。它基于荧光共振能量转移(FRET)和金纳米颗粒的淬灭。选择牛血清白蛋白(BSA)作为模型抗原。异硫氰酸荧光素(FITC)作为FRET供体与抗BSA抗体(anti-BSA–FITC)结合,而BSA与FRET受体与金纳米颗粒(GNPs–BSA)结合。抗BSA–BSA免疫复合物的形成导致抗BSA–FITC和GNPs–BSA之间的FRET。因此,FRET供体的荧光被猝灭,并且降低的荧光强度在线性范围内对受体的浓度线性响应。我们根据BSA与GNP之间的化学计量比获得了BSA的浓度。通过这种方法,我们能够专门检测BSA。 BSA的检出限为0.5 nM,测定的线性范围为2.9-43.5 nM。它已成功应用于血清样品中BSA的特异性检测。

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