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采用加工蛋抗体和加标方法对食物中的卵类过敏原进行定量检测。

Enhanced quantitation of egg allergen in foods using incurred standards and antibodies against processed egg in a model ELISA.

机构信息

Center for Food Safety and Applied Nutrition, United States Food and Drug Administration, 8301 Muirkirk Road, Laurel, MD, 20708, United States.

Center for Food Safety and Applied Nutrition, United States Food and Drug Administration, 5100 Paint Branch Parkway, College Park, MD, 20740, USA.

出版信息

Anal Chim Acta. 2019 Nov 12;1081:157-167. doi: 10.1016/j.aca.2019.07.030. Epub 2019 Jul 19.

DOI:10.1016/j.aca.2019.07.030
PMID:31446953
Abstract

Underestimation of egg allergen from processed foods prompted the evaluation of critical Enzyme-Linked Immunosorbent Assay (ELISA) parameters: (1) extraction of egg proteins from a processed matrix; (2) use of anti-heat processed egg antibodies (Abs) on detectability of modified proteins, and (3) utilization of incurred material as standards. The relative affinity of two combinations of raw (R), boiled (B) and fried (F) Abs to unprocessed/processed egg proteins with or without matrix was determined from antibody (Ab) binding curves. In ELISAs using RBF-Abs and BF-Abs, denaturing buffer, and incurred standards, the Limit of Detection (LOD) and Limit of Quantitation (LOQ) were 0.47 and 0.25; and 1.58 and 0.85, respectively, and the linear range was 0-24 μg g egg protein. The recoveries of egg protein from cookies, cereal bar, and muffin (incurred levels 4.8-48 μg g) with the developed ELISAs were in an acceptable range (50-130%). These ELISAs consistently detected more declared/undeclared egg proteins in market samples compared to assays using PBS for extraction. Overall, better assay performance was observed using BF-Abs. An ELISA combining anti-processed egg Abs, denaturing buffer, and incurred standards promises improved quantitation of egg proteins in processed foods.

摘要

加工食品中鸡蛋过敏原含量被低估,促使人们对关键酶联免疫吸附试验(ELISA)参数进行评估:(1)从加工基质中提取鸡蛋蛋白;(2)使用抗热加工鸡蛋抗体(Abs)检测修饰蛋白的可检测性;(3)利用实际材料作为标准。通过抗体(Ab)结合曲线确定了生(R)、煮(B)和炸(F)Abs 对未加工/加工鸡蛋蛋白与基质结合或不结合的相对亲和力。在使用 RBF-Abs 和 BF-Abs、变性缓冲液和实际标准的 ELISA 中,检测限(LOD)和定量限(LOQ)分别为 0.47 和 0.25;1.58 和 0.85,线性范围为 0-24μg g 鸡蛋蛋白。用开发的 ELISA 从曲奇、谷物棒和松饼(实际含量为 4.8-48μg g)中回收的鸡蛋蛋白回收率在可接受范围内(50-130%)。与使用 PBS 提取相比,这些 ELISA 一致地检测到市场样品中更多申报/未申报的鸡蛋蛋白。总体而言,使用 BF-Abs 可以提高检测性能。结合抗加工鸡蛋 Abs、变性缓冲液和实际标准的 ELISA 有望改善加工食品中鸡蛋蛋白的定量。

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