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Development and evaluation of a real-time PCR assay for detection of lobster, a crustacean shellfish allergen

机译:用于检测龙虾(甲壳类贝类过敏原)的实时PCR分析方法的开发和评估

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摘要

Crustacean shellfish are a leading cause of food allergy in American adults, and the Food Allergen Labeling and Consumer Protection Act requires that different types of crustacean shellfish be distinguished from each other. In general ELISA assays are not capable of differentiating crustacean type, but PCR assays are. In this work, a real-time PCR assay for lobster, a crustacean shellfish allergen, was developed and evaluated. Food matrices were spiked with lobster meat at 0.1, 1, 10, 100, 1000, 10(4), and 10(5) parts per million (ppm). In addition to testing of several different food matrices, method performance was determined using conditions which have historically proven challenging for PCR analyses, specifically food matrices with low DNA content and acidic pH levels, as well as foods that were treated with combined high temperature and pressure. Real-time PCR standard curves were generated from spiked, treated foods and analyzed with respect to linear range and reaction efficiency. In most cases, the assay was linear over 6-8 orders of magnitude; lower limits of detection were 0.1-1 ppm and reaction efficiencies were within the preferred range of 100 +/- 10%. A notable exception occurred in the case of heat treatment at acidic pH, which resulted in severe delay or complete loss of amplification signals. Published by Elsevier Ltd.
机译:甲壳类贝类是美国成年人食物过敏的主要原因,《食品过敏原标签和消费者保护法》要求区分不同类型的甲壳类贝类。通常,ELISA分析不能区分甲壳类,但PCR分析可以。在这项工作中,开发并评估了龙虾(甲壳类贝类过敏原)的实时PCR检测方法。将食品基质中的龙虾肉加标为百万分之一(ppm)0.1、1、10、100、1000、10(4)和10(5)。除了测试几种不同的食品基质外,还使用历史上证明对PCR分析具有挑战性的条件(尤其是低DNA含量和酸性pH值的食品基质以及经高温高压处理的食品)确定了方法的性能。 。从加标处理过的食品中生成实时PCR标准曲线,并就线性范围和反应效率进行分析。在大多数情况下,该分析在6-8个数量级上是线性的。最低检测限为0.1-1 ppm,反应效率在100 +/- 10%的优选范围内。在酸性pH下进行热处理时,有一个明显的例外,这会导致严重的延迟或扩增信号的完全丧失。由Elsevier Ltd.发布

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