Rapid determination of aflatoxin B1 by an automated immunomagnetic bead purification sample pretreatment method combined with high‐performance liquid chromatography

Zhang, Bo; Yu, Leitao; Liu, Zhenjiang; Lu, Hongyang; Fu, Xiaoling; Du, Daolin

doi:10.1002/jssc.202000293

Cited by 11 publications

(2 citation statements)

References 34 publications

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“…The supernatant was collected by centrifugation at 6,000 rpm for 10 min. Fat, protein, pigment, and carbohydrate in the extraction solution were removed by a solid-phase column for AF purification ( Zhang et al, 2020 ). AFB 1 detection was performed by the HPLC method using the following parameters: a mobile phase of 4:6 methanol–water, C18 reversed-phase column with a UV detector, a detection wavelength of 365 nm, and a flow rate of 0.6 ml/min.…”

Section: Methodsmentioning

confidence: 99%

Characterization of a Trametes versicolor aflatoxin B1-degrading enzyme (TV-AFB1D) and its application in the AFB1 degradation of contaminated rice in situ

Yang

Xiao²,

Shen³

et al. 2022

Front. Microbiol.

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Aflatoxin B1 (AFB1) contaminates rice during harvest or storage and causes a considerable risk to human and animal health. In this study, Trametes versicolor AFB1–degrading enzyme (TV–AFB1D) gene recombinantly expressed in engineered E. coli BL21 (DE3) and Saccharomyces cerevisiae. The TV–AFB1D enzymatic characteristics and AFB1 degradation efficiency in contaminated rice were investigated. Results showed that the size of recombinant TV-AFB1D expressing in E. coli BL21 (DE3) and S. cerevisiae was appropriately 77 KDa. The kinetic equation of TV-AFB1D was y = 0.01671x + 1.80756 (R2 = 0.994, Km = 9.24 mM, and Vmax = 553.23 mM/min). The Kcat and Kcat/Km values of TV-AFB1D were 0.07392 (s−1) and 8 M−1 s−1, respectively. The AFB1 concentration of contaminated rice decreased from 100 μg/ml to 32.6 μg/ml after treatment at 32°C for 5 h under the catabolism of TV-AFB1D. S. cerevisiae engineered strains carrying aldehyde oxidase 1 (AOX1) and Cauliflower mosaic virus 35 S (CaMV 35 S) promoters caused the residual AFB1 contents, respectively, decreased to 3.4 and 2.9 μg/g from the initial AFB1 content of 7.4 μg/g after 24 h of fermentation using AFB1-contaminated rice as substrate. The AFB1 degradation rates of S. cerevisiae engineered strains carrying AOX1 and CaMV promoters were 54 and 61%, respectively. Engineered S. cerevisiae strains integrated with TV-AFB1D expression cassettes were developed to simultaneously degrade AFB1 and produce ethanol using AFB1-contaminated rice as substrate. Thus, TV-AFB1D has significant application potential in the AFB1 decomposition from contaminated agricultural products.

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Section: Methodsmentioning

confidence: 99%

Characterization of a Trametes versicolor aflatoxin B1-degrading enzyme (TV-AFB1D) and its application in the AFB1 degradation of contaminated rice in situ

Yang

Xiao²,

Shen³

et al. 2022

Front. Microbiol.

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show abstract

“…The Chinese national standards specifics a maximum limit of less than 20 μg/kg in food in corn, corn flakes, and corn products. The common laboratory methods for detecting AFB1 are immunochromatography (Liu et al, 2020), chemiluminescence (Shim et al, 2014), high‐performance liquid chromatography (Zhang et al, 2020), chromatography–mass spectrometry (Dong et al, 2018), and so on (Qu et al, 2021). However, these approaches are time‐consuming and expensive and require sample preparation and trained personnel to operate the instruments.…”

Section: Introductionmentioning

confidence: 99%

Detection of AFB1 in corn by MXene paper‐based unlabeled aptasensor

Wang,

Gu,

Rong

et al. 2024

J Food Process Engineering

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In this work, a paper‐based electrochemical aptamer sensor was developed for the detection of aflatoxin B1 (AFB1) using a combination of MXene–Ti3C2Tx and nucleic acid aptamers. The prepared single‐layer or few‐layer MXene suspension is suction‐filtered onto MXene paper, which is cut to prepare MXene electrodes. To accomplish AFB1 specific detection, an amino‐labeled AFB1 aptamer is mounted on the surface of the carboxy‐functionalized MXene electrode. When AFB1 is present, it particularly binds to the aptamer to form a 3D structure, reducing the efficiency of electron transmission on the sensor surface. The difference in impedance signal change at the electrode/electrolyte interface is used to quantify AFB1. The results indicated that the detection range is 0.05–100 ng/mL, the detection limit is 0.04 ng/mL, and the recovery rate of AFB1 in corn samples is 97.8%–111.52% with the optimal detection conditions. The MXene paper‐based label‐free aptasensor is versatile and can detect different targets by simply swapping out the aptamers of different targets. The sensor also has a wide range of applications in food analysis and environmental testing.Practical applicationsA paper‐based electrochemical aptamer sensor was developed to detect aflatoxin B1 using a combination of MXene–Ti3C2Tx and nucleic acid aptamers.The design is based on the preparation of MXene electrodes by pumping and filtering monolayer or multilayer MXene suspensions onto MXene paper and cutting.The MXene paper‐based label‐free aptamer sensor was designed to be versatile, allowing the detection of different targets by simply replacing the aptamer with one from a different targets.

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Establishment, application and comparison of three immunoaffinity pretreatment techniques for mycotoxins systematically

Tian,

Liu,

Sun

et al. 2024

Food Measure

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Rapid determination of aflatoxin B1 by an automated immunomagnetic bead purification sample pretreatment method combined with high‐performance liquid chromatography

Cited by 11 publications

References 34 publications

Characterization of a Trametes versicolor aflatoxin B1-degrading enzyme (TV-AFB1D) and its application in the AFB1 degradation of contaminated rice in situ

Characterization of a Trametes versicolor aflatoxin B1-degrading enzyme (TV-AFB1D) and its application in the AFB1 degradation of contaminated rice in situ

Detection of AFB1 in corn by MXene paper‐based unlabeled aptasensor

Establishment, application and comparison of three immunoaffinity pretreatment techniques for mycotoxins systematically

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