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鉴定由溶菌酶和β-乳球蛋白稳定的油水界面中的唾液蛋白。

Identification of salivary proteins at oil-water interfaces stabilized by lysozyme and beta-lactoglobulin.

机构信息

Top Institute Food and Nutrition PO Box 557, 6700 AN Wageningen, The Netherlands.

出版信息

Arch Oral Biol. 2010 Apr;55(4):268-78. doi: 10.1016/j.archoralbio.2010.02.004. Epub 2010 Mar 1.

DOI:10.1016/j.archoralbio.2010.02.004
PMID:20197185
Abstract

In this research, we investigated the interaction occurring between oil-in-water emulsion droplets, stabilized by different emulsifiers, i.e. lysozyme and beta-lactoglobulin (beta-lg), and salivary proteins (SPs) with a molecular mass (M(r)) above about 10kDa. Different techniques, i.e. infrared spectroscopy, Western blotting, PAS staining and SDS-PAGE coupled to MS, were employed for this purpose. This study demonstrated the interaction between several salivary proteins and the emulsifiers at the oil-water interfaces. In particular, results show that the high M(r) mucin MUC5B was strongly bound to lysozyme stabilized emulsions, whereas beta-lg stabilized emulsions associated with MUC7 and, moderately, with MUC5B. Furthermore, we observed that salivary proteins in the range M(r) 10-100kDa associated differently with emulsion droplets. A large majority of SPs was found to interact with lysozyme stabilized emulsion droplets whilst in case of beta-lg stabilized emulsions, the SPs distribute more evenly between the fraction associated and non-associated with the droplets. A clear example is alpha-amylase (M(r) approximately 55kDa) which predominantly associates with lysozyme stabilized emulsion droplets, but not with beta-lg emulsion droplets. To conclude, our findings indicate that adsorption/association of salivary protein components onto the emulsion droplets is related to the type of emulsifying proteins at the oil-water interfaces and it is probably driven by the overall net charge at the droplet's oil-water interfaces, i.e. positive for lysozyme stabilized emulsions and negative for beta-lactoglobulin stabilized emulsion at neutral pH.

摘要

在这项研究中,我们研究了不同乳化剂(即溶菌酶和β-乳球蛋白(β-lg))稳定的油包水乳滴与分子量(Mr)大于约 10kDa 的唾液蛋白(SP)之间的相互作用。为此,采用了不同的技术,即红外光谱、Western 印迹、PAS 染色和 SDS-PAGE 结合 MS。这项研究表明了几种唾液蛋白与油水界面处的乳化剂之间的相互作用。特别是,结果表明,高 Mr 黏液素 MUC5B 与溶菌酶稳定的乳液强烈结合,而β-lg 稳定的乳液与 MUC7 结合,并适度与 MUC5B 结合。此外,我们观察到,分子量在 10-100kDa 范围内的唾液蛋白与乳液滴的结合方式不同。发现大多数 SPs 与溶菌酶稳定的乳液滴相互作用,而对于β-lg 稳定的乳液,SPs 在与乳液滴相关的和不相关的两个部分之间分布更均匀。一个明显的例子是α-淀粉酶(Mr 约 55kDa),它主要与溶菌酶稳定的乳液滴结合,但不与β-lg 乳液滴结合。总之,我们的研究结果表明,唾液蛋白成分在乳液滴上的吸附/结合与油水界面处乳化蛋白的类型有关,并且可能是由乳液滴油-水界面上的总净电荷驱动的,即在中性 pH 下,溶菌酶稳定的乳液带正电荷,而β-乳球蛋白稳定的乳液带负电荷。

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