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Biosensor-Based Screening Method for the Detection of Aflatoxins B_(1)-G_(1)

机译:基于生物传感器的黄曲霉毒素B_(1)-G_(1)检测方法

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Aflatoxins are extremely toxic metabolites from Aspergillus species that can adulterate a wide range of human foodstuff. Herein, we propose a novel assay designed as an analytical test for aflatoxin B_(1) and G_(1) (AFB_(1) and AFG_(1), respectively) that could represent an alternative screening technique for this class of mycotoxins. The approach for the determination of these toxins is based on surface plasmon resonance using neutrophil porcine elastase as a "bait" for these aflatoxins. The selection and optimization of the analytical procedure involved a preliminary investigation on the type of inhibition by AFB_(1): the level of the protease inhibition exerted by AFB_(1) depended upon the incubation time and the concentration of the binding partners, showing the competitiveness and the reversibility of the inhibition. A posteriori, the nature of the interaction granted a rapid analysis, a single detection test requiring only a few minutes. For the development of the assay, the experimental conditions were evaluated and optimized with both calibration solution and aflatoxin-spiked samples. To apply this method to aflatoxin-contaminated maize, a rapid solid-phase extraction treatment was developed. The proposed assay for AFB_(1) and AFG_(1) was validated by comparison with both a chromatographic reference method and a standard enzyme linked immunosorbent assay procedure. This enzyme-based biosensor represents a new approach for the detection of aflatoxins based on the reversible interaction between a blocked macromolecule and a soluble ligand, having the major advantages in the relative rapidity, the reusability of the capturing surface, and low cost per single test.
机译:黄曲霉毒素是曲霉属物种的剧毒代谢产物,可掺入多种人类食品。在本文中,我们提出了一种新颖的测定方法,该方法设计为黄曲霉毒素B_(1)和G_(1)(分别为AFB_(1)和AFG_(1))的分析测试,可以代表此类真菌毒素的替代筛选技术。确定这些毒素的方法是基于表面等离振子共振,使用中性粒细胞猪弹性蛋白酶作为这些黄曲霉毒素的“诱饵”。分析程序的选择和优化涉及对AFB_(1)抑制类型的初步研究:AFB_(1)发挥的蛋白酶抑制水平取决于孵育时间和结合伴侣的浓度,显示了竞争力和可逆性的抑制。后验,相互作用的性质可以进行快速分析,一次检测只需几分钟。为了开发测定方法,使用校准溶液和加有黄曲霉毒素的样品对实验条件进行了评估和优化。为了将该方法应用于受黄曲霉毒素污染的玉米,开发了一种快速固相萃取处理方法。通过与色谱参考方法和标准酶联免疫吸附测定程序进行比较,验证了针对AFB_(1)和AFG_(1)提出的测定方法。这种基于酶的生物传感器代表了一种基于封闭大分子与可溶性配体之间可逆相互作用的黄曲霉毒素检测新方法,其主要优点是相对快速,捕获表面的可重复使用性以及每次测试的低成本。

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