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通过监测酪蛋白特征性肽实现牛奶种属特异性分析。

Toward milk speciation through the monitoring of casein proteotypic peptides.

机构信息

Dipartimento di Scienza degli Alimenti - Università di Napoli 'Federico II', Parco Gussone, 80055 Portici (Napoli), Italy.

出版信息

Rapid Commun Mass Spectrom. 2010 Jun 15;24(11):1687-96. doi: 10.1002/rcm.4564.

DOI:10.1002/rcm.4564
PMID:20486267
Abstract

The possibility of detecting extraneous milk in singles species cheese-milk has been explored. A mass spectrometry (MS)-based procedure has been developed to detect 'signature peptides', corresponding to the predefined subset of 'proteotypic peptides', as matchless analytical surrogates of the parent caseins. Tryptic digests of skimmed milk samples from four species were analyzed by matrix-assisted laser desorption/ionization time-of-flight (MALDI-TOF) MS. Amongst the candidate signature peptides that are able to differentiate milks from the four species, the alpha(s1)-casein (CN) f8-22 peptide was selected as a convenient marker for bovine, ovine and water buffalo milk while the f4-22 peptide was selected as a marker for the two caprine alpha(s1)-CN A and B variants, which differ by a Pro(16) (B)->Leu(16) (A) substitution. MALDI analysis of the digest allowed the detection of alpha(s1)-CN f8-22 and caprine alpha(s1)-CN f4-22. The accurate evaluation of caprine milk in a quaternary mixture required the development of a liquid chromatography/electrospray ionization (LC/ESI)-MS procedure. Five synthetic signature peptide analogues, which differed from their natural counterparts by a single amino acid substitution, were used as internal standards to quantify the alpha(s1)-CN, which was chosen as a reference milk protein, from the different species. The limits of detection were 0.5% (1% for caprine) for either the MALDI or the LC/ESI-MS method. The isotopic-label-free quantification of isoform- or variant-specific signature peptides has disclosed a convenient approach for targeting proteins in complex mixtures.

摘要

已经探索了在单一物种奶酪乳中检测外来乳的可能性。已经开发了一种基于质谱 (MS) 的程序来检测“特征肽”,这些特征肽对应于“蛋白质特征肽”的预定义子集,是原始酪蛋白的无与伦比的分析替代物。对来自四个物种的脱脂奶样品的胰蛋白酶消化物进行了基质辅助激光解吸/电离飞行时间 (MALDI-TOF) MS 分析。在所能够区分四个物种牛奶的候选特征肽中,选择了 alpha(s1)-酪蛋白 (CN) f8-22 肽作为牛、羊和水牛奶的方便标记物,而 f4-22 肽被选为两种山羊 alpha(s1)-CN A 和 B 变体的标记物,这两种变体在 Pro(16) (B) 取代为 Leu(16) (A)。消化物的 MALDI 分析允许检测到 alpha(s1)-CN f8-22 和山羊 alpha(s1)-CN f4-22。在四元混合物中准确评估山羊奶需要开发液相色谱/电喷雾电离 (LC/ESI)-MS 程序。使用了五个合成特征肽类似物,它们与天然对应物仅相差一个氨基酸取代,用作内部标准来定量不同物种的 alpha(s1)-CN,alpha(s1)-CN 被选为参考乳蛋白。MALDI 或 LC/ESI-MS 方法的检测限均为 0.5%(山羊为 1%)。无同位素标记的同种型或变体特异性特征肽的定量已经揭示了一种针对复杂混合物中蛋白质的便捷方法。

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