Affinity capture of aflatoxin B1 and B2 by aptamer-functionalized magnetic agarose microspheres prior to their determination by HPLC

被引:0
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作者
Hongmei Liu
Anxiang Lu
Hailong Fu
Bingru Li
Meihua Yang
Jihua Wang
Yunxia Luan
机构
[1] Beijing Research Center for Agricultural Standards and Testing,Key Laboratory of Bioactive Substances and Resources Utilization of Chinese Herbal Medicine, Ministry of Education, Institute of Medicinal Plant Development
[2] Agricultural Product Quality and Safety Risk Assessment Laboratory of the Department of Agriculture,undefined
[3] Beijing Municipal Key Laboratory of Agriculture Environment Monitoring,undefined
[4] Chinese Academy of Medical Sciences & Peking Union Medical College,undefined
来源
Microchimica Acta | 2018年 / 185卷
关键词
Oligonucleotide; Aptamer; Aflatoxin B; Aflatoxin B; Mycotoxin; Magnetic agarose microspheres; Biotin–streptavidin system; Magnetic solid-phase extraction; HPLC-PCD-FLD; Maize;
D O I
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中图分类号
学科分类号
摘要
A novel adsorbent is described for magnetic solid-phase extraction (MSPE) of the aflatoxins AFB1 and AFB2 (AFBs). Magnetic agarose microspheres (MAMs) were functionalized with an aptamer to bind the AFBs which then were quantified by HPLC and on-line post-column photochemical derivatization with fluorescence detection. Streptavidin-conjugated MAMs were synthesized first by a highly reproducible strategy. They possess strong magnetism and high surface area. The MAMs were characterized by transmission electron microscopy, scanning electron microscopy, optical microscopy, laser diffraction particle size analyzer, Fourier transform infrared spectrometry, vibrating sample magnetometry and laser scanning confocal microscopy. Then, the AFB-aptamers were immobilized on MAMs through biotin–streptavidin interaction. Finally, the MSPE is performed by suspending the aptamer-modified MAMs in the sample. They are then collected by an external magnetic field and the AFBs are eluted with methanol/buffer (20:80). Several parameters affecting the coupling, capturing and eluting efficiency were optimized. Under the optimized conditions, the method is fast, has good linearity, high selectivity, and sensitivity. The LODs are 25 pg·mL−1 for AFB1 and 10 pg·mL−1 for AFB2. The binding capacity is 350 ± 8 ng·g−1 for AFB1 and 384 ± 8 ng·g−1 for AFB2, and the precision of the assay is <8%. The method was successfully applied to the analysis of AFBs in spiked maize samples.
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