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通过免疫酶法和质谱法对酪蛋白中热诱导乳糖基化产物的表征

Characterization of heat-induced lactosylation products in caseins by immunoenzymatic and mass spectrometric methodologies.

作者信息

Scaloni Andrea, Perillo Valentina, Franco Paolo, Fedele Elena, Froio Raffaele, Ferrara Lino, Bergamo Paolo

机构信息

Proteomics and Mass Spectrometry Laboratory, I.A.B.B.A.M., National Research Council, Naples, Italy.

出版信息

Biochim Biophys Acta. 2002 Jul 29;1598(1-2):30-9. doi: 10.1016/s0167-4838(02)00290-x.

DOI:10.1016/s0167-4838(02)00290-x
PMID:12147341
Abstract

Nonenzymatic glycosylation of proteins occur during milk thermal treatment through the Maillard reaction. Immunoenzymatic and spectrometric methodologies were used to investigate caseins modification in samples submitted to different processing. As expected, protein-bound carbonyl content in raw and thermal-treated milks was positively correlated with the severity of the treatment. When immunoblotting and ELISA experiments were carried out either on isolated or whole milk proteins, carbonyl accumulation on caseins and macromolecular aggregates produced by thermal processing was evidenced. A comparative electrospray-mass spectrometry (ES-MS) analysis of different milks allowed verifying the extent of Amadori adducts on the more abundant protein components (alphas1- and beta-casein (alphas1- and beta-CN)). A combined matrix-assisted laser desorption ionization (MALDI)-MS/Edman degradation approach on enzymatic digests identified caseins modification sites. In moderately heat-treated milks, we observed that lactosylation occurred specifically at Lys-34 (alphas1-CN) and Lys-107 (beta-CN); whereas, samples subjected to more severe conditions presented modification at Lys-7, Lys-34, Lys-83, Lys-103, Lys-105, Lys-132 and Lys-193 (alphas1-CN) and at Lys-32, Lys-48, Lys-107, Lys-113 and Lys-176 (beta-CN). Differences in secondary structure of these components was assayed by circular dichroism (CD) spectroscopy.

摘要

蛋白质的非酶糖基化在牛奶热处理过程中通过美拉德反应发生。采用免疫酶法和光谱法研究了不同加工条件下样品中酪蛋白的修饰情况。正如预期的那样,生牛奶和热处理牛奶中与蛋白质结合的羰基含量与处理的强度呈正相关。当对分离的或全脂牛奶蛋白进行免疫印迹和酶联免疫吸附测定实验时,发现了酪蛋白上的羰基积累以及热处理产生的大分子聚集体。对不同牛奶进行的比较电喷雾质谱(ES-MS)分析,验证了含量较高的蛋白质成分(αs1-酪蛋白和β-酪蛋白(αs1-CN和β-CN))上阿马多里加合物的程度。对酶解产物采用基质辅助激光解吸电离(MALDI)-MS/埃德曼降解相结合的方法,确定了酪蛋白的修饰位点。在适度热处理的牛奶中,我们观察到乳糖基化特异性发生在赖氨酸-34(αs1-CN)和赖氨酸-107(β-CN)处;而在更严格条件下处理的样品中,赖氨酸-7、赖氨酸-34、赖氨酸-83、赖氨酸-103、赖氨酸-105、赖氨酸-132和赖氨酸-193(αs1-CN)以及赖氨酸-32、赖氨酸-48、赖氨酸-107、赖氨酸-113和赖氨酸-176(β-CN)处出现了修饰。通过圆二色性(CD)光谱分析了这些成分二级结构的差异。

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