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基于纳米金的侧向流动免疫分析法用于检测缓冲体系中赭曲霉毒素A的研究进展

Development of nanogold-based lateral flow immunoassay for the detection of ochratoxin A in buffer systems.

作者信息

Moon Jihea, Kim Giyoung, Lee Sangdae

机构信息

Postharvest Engineering Division, Department of Agricultural Engineering, National Academy of Agricultural Sciences, Suwon 441-707, Korea.

出版信息

J Nanosci Nanotechnol. 2013 Nov;13(11):7245-9. doi: 10.1166/jnn.2013.8099.

Abstract

Ochratoxin A (OTA), classified as a possible human renal carcinogen (group 2B), is a potent toxin as to cause the nephropathy. Many methods have been proposed and reviewed for OTA determination in food and agricultural products. However, current analytical procedures of mycotoxin are based on the time-delayed analysis. To reduce the contamination of OTA during distribution and storage of food and feeds, a rapid and easy-to-use detection method is required. The strip assay is an easy and fast detection method that is very reliable and cheap in production. The purpose of this study was to improve the sensitivity of strip sensor by simplifying the manufacturing steps and detection reading. Feasibility of strip assay detection of OTA was determined by color appearance of test line that was produced by the binding between OTA-BSA conjugates and gold antibody particles. However, in this study, strip assays were improved the efficacy of detection by conjugating with nanoparticles and OTA-BSA conjugates, instead of antibody. By different optimization steps in strip manufacturing and the application of the label on the strips, an increase in sensitivity and applicability was accomplished. The method uses a low cost test device consisting of a conjugation pad, membrane, sample pad, and absorbent pad. OTA-BSA and their conjugates with colloidal gold nanoparticles were prepared. The detection was based on the competition of OTA in a sample and an OTA-BSA on the colloidal particle surfaces for the binding to antibody of OTA immobilized on a membrane. It allows direct analysis of sample containing 10% methanol in phosphate buffered saline. The limit of detection obtained was 10 ng/ml for OTA. The cross reactivity of OTA strip assays with Aflatoxin B1 (AFB1) was examined. When 10, 100 ng/ml of AFB1 was tested, non-specific binding was not observed in the test strip.

摘要

赭曲霉毒素A(OTA)被归类为可能的人类肾脏致癌物(2B组),是一种可导致肾病的强效毒素。已经提出并综述了许多用于食品和农产品中OTA测定的方法。然而,目前霉菌毒素的分析程序基于延时分析。为了减少食品和饲料在分销和储存过程中OTA的污染,需要一种快速且易于使用的检测方法。试纸条检测是一种简单快速的检测方法,在生产中非常可靠且成本低廉。本研究的目的是通过简化制造步骤和检测读数来提高试纸条传感器的灵敏度。通过OTA-BSA偶联物与金抗体颗粒之间的结合产生的测试线的颜色外观来确定试纸条检测OTA的可行性。然而,在本研究中,试纸条检测通过与纳米颗粒和OTA-BSA偶联物而非抗体结合来提高检测效率。通过试纸条制造中的不同优化步骤以及标签在试纸上的应用,实现了灵敏度和适用性的提高。该方法使用由结合垫、膜、样品垫和吸收垫组成的低成本测试装置。制备了OTA-BSA及其与胶体金纳米颗粒的偶联物。检测基于样品中的OTA与胶体颗粒表面的OTA-BSA竞争结合固定在膜上的OTA抗体。它允许直接分析磷酸盐缓冲盐水中含10%甲醇的样品。获得的OTA检测限为10 ng/ml。检测了OTA试纸条检测与黄曲霉毒素B1(AFB1)的交叉反应性。当测试10、100 ng/ml的AFB1时,在试纸条中未观察到非特异性结合。

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