Competitive photometric and visual ELISA for aflatoxin B1 based on the inhibition of the oxidation of ABTS

被引:0
|
作者
Ying Tang
Wenqiang Lai
Jin Zhang
Dianping Tang
机构
[1] Chongqing University of Arts and Sciences,Chongqing Key Laboratory of Environmental Materials & Remediation Technologies
[2] Minnan Normal University,Fujian Provincial Key Laboratory of Modern Analytical Science and Separation Technology, College of Chemistry and Environment
[3] Fuzhou University,MOE Key Laboratory of Analysis and Detection for Food Safety, Department of Chemistry
来源
Microchimica Acta | 2017年 / 184卷
关键词
Colorimetric immunoassay; Single-shot assay; UV-vis adsorption spectroscopy; Cuvette; Microtiter plate; Oxidation-reduction reaction; Enzymatic catalytic reaction; Naturally contaminated/spiked food sample;
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摘要
This work reports on a sensitive colorimetric immunoassay for aflatoxin B1 (AFB1) in foodstuff. The reagent L-ascorbic acid 2-phosphate (AAP) is added to the system, and alkaline phosphatase (ALP) hydrolyzes AAP under formation of ascorbic acid and phosphate. The ascorbic acid produced reduces chloroauric acid to form zero-valent gold (in the form of nanoparticles). Hence, Au(III) is no longer available to oxidize 2,2′-azinobis(3-ethylbenzthiazoline-6-sulfonate) (ABTS) to form a green product. Rather, the solution remains colorless. By using ALP-labelled monoclonal anti-AFB1 antibody, a competitive enzyme-label immunoassay was developed for AFB1 in a microplate coated with the AFB1-BSA conjugate. Under optimal conditions, the absorbance of the solution at 415 nm increases linearly with increasing AFB1 concentration in range from 10 pg·mL−1 to 100 ng·mL−1 (while the color gradually turns to green), and the detection limit is 7.8 pg·mL−1. The precision of the method (expressed as RSD) is ±9.7%. The accuracy was validated by analyzing both naturally contaminated and spiked food samples, and the results matched the results obtained by ELISA very well.
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页码:2387 / 2394
页数:7
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