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基于高发光量子点微球的超高灵敏竞争型荧光免疫分析,用于调节竞争抗原与抗体的亲和力。

Ultrasensitive direct competitive FLISA using highly luminescent quantum dot beads for tuning affinity of competing antigens to antibodies.

机构信息

State Key Laboratory of Food Science and Technology, Nanchang University, Nanchang 330047, PR China.

College of Science, Northwest A&F University, Yangling, Shaanxi 712100, PR China.

出版信息

Anal Chim Acta. 2017 Jun 15;972:94-101. doi: 10.1016/j.aca.2017.03.039. Epub 2017 Mar 30.

DOI:10.1016/j.aca.2017.03.039
PMID:28495100
Abstract

Herein, for the first time we report a novel direct competitive fluorescence-linked immunosorbent assay (dcFLISA) for the ultrasensitive detection of ochratoxin A (OTA) by introducing a large size polymer beads loaded with quantum dots (QBs) as carrier of competing antigen for decreasing binding affinity to antibody and enhancing the fluorescent signal intensity. When using 255 nm QBs as carrier of competing antigen, the equilibrium dissociation constant of QB based competing antigen to antibodies can be tuned to 100 times higher than that of the horseradish peroxidase (HRP) based competing antigen by controlling labeled amounts of antigen on the surface of QBs. Various parameters that influenced the sensitivity of dcFLISA were investigated and optimized. Under optimum detection parameters, the dynamic linear range of developed dcFLISA for detecting OTA was established at 0.05 pg/mL to 1.56 pg/mL with a half maximal inhibitory concentration at 0.14 ± 0.04 pg/mL (n = 5), which is three orders of magnitude lower than that of conventional HRP-based dcELISA (0.24 ng/mL). The developed FLISA is also highly accurate, reliable, and shows no cross reaction to other mycotoxins. In summary, the proposed method offers a straightforward approach to improve the sensitivity of direct competitive immunoassay for trace small chemical molecule detection in food quality control, environmental monitoring, and clinical diagnosis.

摘要

本文首次报道了一种新型的直接竞争荧光免疫分析(dcFLISA)方法,用于超灵敏检测赭曲霉毒素 A(OTA)。该方法通过引入负载量子点(QBs)的大尺寸聚合物珠作为竞争抗原的载体,降低与抗体的结合亲和力并增强荧光信号强度,从而实现了对 OTA 的检测。当使用 255nm 的 QBs 作为竞争抗原的载体时,通过控制 QBs 表面标记的抗原量,可以将基于 QB 的竞争抗原与抗体的平衡解离常数调至高于基于辣根过氧化物酶(HRP)的竞争抗原的 100 倍。研究并优化了影响 dcFLISA 灵敏度的各种参数。在最佳检测参数下,所建立的 dcFLISA 检测 OTA 的动态线性范围为 0.05pg/mL 至 1.56pg/mL,半数抑制浓度为 0.14±0.04pg/mL(n=5),比传统的基于 HRP 的 dcELISA(0.24ng/mL)低三个数量级。该 FLISA 还具有高度的准确性、可靠性,并且与其他霉菌毒素无交叉反应。总之,该方法为提高痕量小分子在食品质量控制、环境监测和临床诊断中的直接竞争免疫分析的灵敏度提供了一种简单的方法。

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