Oriented boronate affinity–imprinted inverse opal hydrogel for glycoprotein assay via colorimetry

被引:0
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作者
Huan Wang
Jie Wang
Yuetong Wang
Yuqin Liu
Rui Liu
Xuelin Wang
Hui Tan
Tianfu Wang
Tiantian Kong
机构
[1] The First Affiliated Hospital,Department of Biomedical Engineering
[2] Shenzhen University,State Key Laboratory of Bioelectronics, School of Biological Science and Medical Engineering
[3] Southeast University,College of Engineering
[4] Nanjing Agricultural University,Department of Genetic Engineering, College of Natural Science
[5] University of Suwon,Department of Neurosurgery
[6] Ulink College of Suzhou Industrial Park,undefined
[7] The First Affiliated Hospital,undefined
[8] Shenzhen University,undefined
来源
Microchimica Acta | 2020年 / 187卷
关键词
Oriented surface molecularly imprinting; Colloidal crystal; Microfluidics; Hydrogel; Large specific surface area; Biomimetic antibody; Label-free detection; ELISA; Optical biosensor;
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学科分类号
摘要
A biomimetic antibody is described for colorimetric determination of glycoprotein, and horseradish peroxidase (HRP) is used as model analyte. Use is made of oriented surface imprinted inverse opal hydrogel particles functionalized with phenylboronic acid. The inverse opal hydrogel particles were negatively replicated from silica colloidal crystal beads (SCCBs), so that they were endowed with larger specific surface area than the bulk structure. Benefit from that, there were abundant surface molecularly imprinting sites in the hydrogel particles. Because the imprinting sites match the structure of the template molecules, they can recognize HRP with high selectivity and sensitivity. The recognized glycoprotein was bonded with the phenylboronic acid within the sites. The bonded HRP was determined by colorimetry of 3, 3′, 5, 5′-tetramethylbenzidine (TMB) single-component solution at 450 nm, and it shows a 16.03 imprinting factor under optimized conditions. Alpha-fetoprotein (AFP) was also investigated and demostrated the value of this strategy in practical applications. The results show that the absorbance increases linearly in the 1–50 ng mL−1 AFP concentration range and has a 1.32 ng mL−1 detection limit. The assay of human serum was realized by the standard addition method. This strategy is promising to open new horizons for glycoprotein assay.
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