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基于液相色谱-质谱检测的食品中乳蛋白定量方法的开发与验证

Development and validation of a method for the quantification of milk proteins in food products based on liquid chromatography with mass spectrometric detection.

作者信息

Lutter Petra, Parisod Véronique, Weymuth Hans

机构信息

Nestle Research Centre, Quality and Safety Department, Vers-chez-les-Blanc, PO Box 44, 1000 Lausanne 26, Switzerland.

出版信息

J AOAC Int. 2011 Jul-Aug;94(4):1043-59.

PMID:21919337
Abstract

The protection of allergic consumers is crucial to the food industry. Therefore, accurate methods for the detection of food allergens are required. Targeted detection of selected molecules by MS combines high selectivity with accurate quantification. A confirmatory method based on LC/selected reaction monitoring (SRM)-MS/MS was established and validated for the quantification of milk traces in food. Tryptic peptides of the major milk proteins beta-lactoglobulin, beta-casein, alphaS2-casein, and K-casein were selected as quantitative markers. Precise quantification was achieved using internal standard peptides containing isotopically labeled amino acids. For each peptide, qualifier and quantifier fragments were selected according to Commission Decision 2002/657/EC. A simple sample preparation method was established without immunoaffinity or SPE enrichment steps for food matrixes containing different amounts of protein, such as baby food, breakfast cereals, infant formula, and cereals. Intermediate reproducibility, repeatability, accuracy, and measurement uncertainty were determined for each matrix. LOD values of 0.2-0.5 mg/kg, e.g., for beta-lactoglobulin, were comparable to those obtained with ELISA kits. An LOQ of approximately 5 mg/kg, expressed as mass fraction skim milk powder, was validated in protein-rich infant cereals. The obtained validation data show that the described LC/SRM-MS/MS approach can serve as a confirmatory method for the determination of milk traces in selected food matrixes.

摘要

保护过敏体质的消费者对食品行业至关重要。因此,需要准确的食品过敏原检测方法。通过质谱对选定分子进行靶向检测,兼具高选择性和准确定量。建立了一种基于液相色谱/选择反应监测(SRM)-串联质谱的确证方法,并对食品中痕量牛奶的定量进行了验证。选择了主要牛奶蛋白β-乳球蛋白、β-酪蛋白、αS2-酪蛋白和κ-酪蛋白的胰蛋白酶肽段作为定量标志物。使用含有同位素标记氨基酸的内标肽段实现了精确定量。对于每个肽段,根据欧盟委员会第2002/657/EC号决定选择定性和定量碎片。建立了一种简单的样品制备方法,无需免疫亲和或固相萃取富集步骤,适用于含有不同蛋白质含量的食品基质,如婴儿食品、早餐谷物、婴儿配方奶粉和谷物。测定了每种基质的中间精密度、重复性、准确性和测量不确定度。例如,β-乳球蛋白的检测限为0.2-0.5 mg/kg,与酶联免疫吸附测定试剂盒的结果相当。以脱脂奶粉质量分数表示的约5 mg/kg的定量限在富含蛋白质的婴儿谷物中得到验证。所获得的验证数据表明,所述液相色谱/选择反应监测-串联质谱方法可作为选定食品基质中痕量牛奶测定的确证方法。

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