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基于凝乳酶诱导分离、等电沉淀或超速离心制备的干酪素和乳清的比较蛋白质组学分析。

Comparative proteomic analysis of casein and whey as prepared by chymosin-induced separation, isoelectric precipitation or ultracentrifugation.

机构信息

Department of Food Science, Aarhus University, DK-8830 Tjele, Denmark.

出版信息

J Dairy Res. 2012 Nov;79(4):451-8. doi: 10.1017/S0022029912000404. Epub 2012 Sep 24.

DOI:10.1017/S0022029912000404
PMID:22998726
Abstract

Fractionation of bovine milk was performed using chymosin-induced separation, isoelectric precipitation or ultracentrifugation as separation techniques prior to gel-based proteomic analysis. This approach allowed for comparative display and identification of proteins partitioned into casein and whey, respectively. Initially, three different staining methods (silver staining, colloidal Coomassie Blue G-250 or fluorescent Flamingo Pink staining) for two-dimensional gel electrophoresis (2-DGE) analysis were compared for their suitability as staining agent, especially in relation to their suitability to reveal differences in the casein fractions. Fluorescent staining proved to be the most appropriate for this purpose, giving a high sensitivity, and using this staining method, characteristic 2-DGE fingerprints were obtained for each casein and whey fraction from each separation method. A number of protein spots in both casein and whey fractions varied with separation method and these spots were subsequently identified using tandem mass spectrometry (MS). In rennet casein, proteolytic fragmentation of caseins (α(s1)-, α(s2),-, β- and κ-) was identified as a result of chymosin hydrolysis, whereas the 2-DGE profile of acid and ultracentrifuged casein was dominated by the presence of multiple isoforms of κ-caseins. Furthermore, casein remnants were identified in milk serum after ultracentrifugation. This study shows that gel-based proteomic analysis is suitable for characterisation of subtle variations in protein composition of milk fractions that occur as a consequence of different milk fractionation strategies.

摘要

采用凝乳酶诱导分离、等电沉淀或超速离心作为分离技术对牛乳进行分级,然后进行凝胶蛋白质组学分析。这种方法允许对分别分配到酪蛋白和乳清中的蛋白质进行比较显示和鉴定。最初,比较了三种不同的染色方法(银染、胶体考马斯亮蓝 G-250 或荧光 Flamingo Pink 染色)用于二维凝胶电泳(2-DGE)分析,以评估其作为染色剂的适用性,特别是在适合揭示酪蛋白部分差异方面。荧光染色证明最适合这种目的,具有很高的灵敏度,并且使用这种染色方法,从每种分离方法获得了每个酪蛋白和乳清部分的特征 2-DGE 指纹图谱。在凝乳酶酪蛋白中,由于凝乳酶水解,酪蛋白(α(s1)-、α(s2)-、β-和 κ-)发生蛋白水解片段化,而酸和超速离心酪蛋白的 2-DGE 图谱主要由κ-酪蛋白的多种同工型存在。此外,在超离心乳清后,在乳清血清中鉴定到酪蛋白残余物。本研究表明,基于凝胶的蛋白质组学分析适合于表征由于不同的乳分馏策略而导致的乳分馏中蛋白质组成的细微变化。

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