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酶联免疫吸附法检测食品中的核桃残留。

Detection of walnut residues in foods using an enzyme-linked immunosorbent assay.

机构信息

Food Allergy Research & Resource Program, Dept. of Food Science and Technology, Univ. of Nebraska-Lincoln, Lincoln, NE 68583-0919, USA.

出版信息

J Food Sci. 2009 Aug;74(6):T51-7. doi: 10.1111/j.1750-3841.2009.01214.x.

DOI:10.1111/j.1750-3841.2009.01214.x
PMID:19723237
Abstract

Tree nuts, including walnuts, can be responsible for allergic reactions. Food manufacturers have the responsibility to declare the presence of walnuts on packaged foods even when trace residues may be present from the use of shared equipment or the adventitious contamination of ingredients. The aim of this study was to develop a rapid, sensitive, and specific enzyme-linked immunosorbent assay (ELISA) method for the detection of walnut protein residues. Mixtures of raw and roasted English walnuts of several varieties were defatted, powdered, and used as separate antigens in sheep and New Zealand white rabbits. An ELISA was developed using the sheep antiroasted walnut serum as the capture reagent and rabbit antiroasted walnut serum as the detector reagent followed by addition of commercial goat anti-rabbit IgG antibody labeled with alkaline phosphatase and subsequent substrate addition. The performance of the ELISA was validated by testing known amounts of walnut (0 to 100 ppm) either spiked into or manufactured into milk chocolate, cookies, muffins, or ice cream. Recoveries of 1 to 100 ppm walnut-in-chocolate ranged from 71.6% to 119%+/- 7% to 16.5%. The walnut ELISA has a detection limit of 1 ppm (1 microg/g) walnut in several food matrices. Substantial cross-reactivity was observed with pecan while minimal cross-reactivity was noted for hazelnut, mustard, mace, and poppy seed among almost 100 foods and food ingredients tested. This walnut ELISA can be used to detect undeclared walnut residues in foods and ingredients and as a tool to validate the effectiveness of allergen control programs for walnuts.

摘要

树坚果,包括核桃,可能会引起过敏反应。食品制造商有责任在包装食品上声明核桃的存在,即使微量残留可能来自于使用共享设备或成分偶然污染。本研究的目的是开发一种快速、灵敏、特异的酶联免疫吸附测定(ELISA)方法来检测核桃蛋白残留。几种品种的生核桃和烤核桃混合物脱脂、粉碎,分别作为绵羊和新西兰白兔的抗原。使用绵羊抗烤核桃血清作为捕获试剂,兔抗烤核桃血清作为检测试剂,建立 ELISA,随后加入商业山羊抗兔 IgG 抗体,标记碱性磷酸酶,再加入底物。通过测试已知量(0 至 100ppm)的核桃,无论是添加到牛奶巧克力、饼干、松饼还是冰淇淋中,还是在制造过程中添加到这些食品中,验证了 ELISA 的性能。在巧克力中添加 1 至 100ppm 核桃的回收率在 71.6%至 119%+/-7%至 16.5%之间。该核桃 ELISA 在几种食品基质中的检测限为 1ppm(1μg/g)核桃。在测试的近 100 种食品和食品成分中,与山核桃相比,该 ELISA 对美洲山核桃表现出显著的交叉反应性,而对榛子、芥末、肉豆蔻和罂粟籽的交叉反应性最小。该核桃 ELISA 可用于检测食品和成分中未申报的核桃残留,并可作为验证针对核桃的过敏原控制计划有效性的工具。

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