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A Gold Nanoparticle and Aflatoxin B1-BSA Conjugates Based Lateral Flow Assay Method for the Analysis of Aflatoxin B1

机译:一种金纳米颗粒和黄曲霉毒素B1-BSA结合的横向流动分析方法用于分析黄曲霉毒素B1

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摘要

A rapid and simple immuno-chromatographic assay was developed to detect aflatoxin B1 (AFB1). The assay was based on a modified competitive binding format using colloidal gold and polyclonal antibody (Pab) conjugates. The anti-AFB1 Pab was immobilized to a defined detection zone on a porous nitrocellulose membrane and colloidal gold particles were conjugated to AFB1-BSA which served as a detection reagent. The AFB1-containing sample was added to the membrane and allowed to move with AFB1-BSA-coated particles dried on the conjugation pad. The mixture was then passed along the porous membrane by capillary action past the Pab in the detection zone, which captured AFB1 or AFB1-BSA. AFB1 in the sample inhibits binding of AFB1-BSA conjugated gold particles to the Pab and prevents formation of a red color dot. In the absence of AFB1, AFB1-BSA conjugated gold particles bound to the Pab, give a red color within this detection zone. With this method, 10 μg/mL of AFB1 was detected in less than 10 min. The developed AFB1 assay also showed no cross reaction to Ochratoxin A (OTA).
机译:建立了一种快速,简单的免疫色谱分析方法来检测黄曲霉毒素B1(AFB1)。该测定基于使用胶体金和多克隆抗体(Pab)缀合物的改良竞争结合形式。将抗AFB1 Pab固定在多孔硝化纤维素膜上的特定检测区域,并将胶体金颗粒与用作检测试剂的AFB1-BSA偶联。将含有AFB1的样品添加到膜中,并使其与在共轭垫上干燥的AFB1-BSA涂层的颗粒一起移动。然后通过毛细管作用使混合物沿着多孔膜通过检测区域中的Pab,该区域捕获了AFB1或AFB1-BSA。样品中的AFB1抑制了AFB1-BSA共轭金颗粒与Pab的结合,并防止了红色斑点的形成。在没有AFB1的情况下,结合到Pab的AFB1-BSA共轭金颗粒在该检测区内呈红色。使用此方法,在不到10分钟的时间内检测到10μg/ mL的AFB1。发达的AFB1测定法也未发现与O曲霉毒素A(OTA)的交叉反应。

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