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超滤过程中牛血清白蛋白聚集的机制。

Mechanism of bovine serum albumin aggregation during ultrafiltration.

作者信息

Maruyama T, Katoh S, Nakajima M, Nabetani H

机构信息

National Food Research Institute, Kannondai 2-1-2, Tsukuba, Ibaraki, Japan 305-8642.

出版信息

Biotechnol Bioeng. 2001 Oct 20;75(2):233-8. doi: 10.1002/bit.10001.

DOI:10.1002/bit.10001
PMID:11536147
Abstract

Protein fouling is a critical problem for ultrafiltration. In this study, we adopted bovine serum albumin (BSA) as a model protein and polysulfone membrane as a typical ultrafiltration membrane. We then investigated the factors of the protein denaturation and aggregation, such as stirring shear stress and intermolecular exchange of disulfide during ultrafiltration, and discussed the BSA fouling mechanism. Fourier transform-infrared analysis revealed that magnetic stirring did not cause any difference in the secondary structural change of BSA gel-like deposits on the ultrafiltration membrane. BSA aggregates were collected from BSA gel-like deposits on the ultrafiltration membrane by centrifugation. Polyacrylamide gel electrophoresis in SDS analysis of BSA aggregates proved that the major binding of the BSA aggregates involved intermolecular disulfhydryl binding and that capping the free thiol group in BSA molecules with cysteine induced a remarkable decrease in the amount of the BSA aggregates during ultrafiltration. We concluded that one of the main factors in the BSA aggregation during ultrafiltration is the intermolecular exchange of disulfide through cysteinyl residue. We also found that the BSA aggregation caused a decrease in alpha-helix from 66% to 50% and an increase in beta-sheet from 20% to 36%, which was presumably because the cysteine residues associated with the intermolecular disulfide bonds had been located in alpha-helices.

摘要

蛋白质污染是超滤过程中的一个关键问题。在本研究中,我们采用牛血清白蛋白(BSA)作为模型蛋白,聚砜膜作为典型的超滤膜。然后,我们研究了超滤过程中蛋白质变性和聚集的因素,如搅拌剪切应力和二硫键的分子间交换,并探讨了BSA的污染机制。傅里叶变换红外分析表明,磁力搅拌不会导致超滤膜上BSA凝胶状沉积物的二级结构变化出现任何差异。通过离心从超滤膜上的BSA凝胶状沉积物中收集BSA聚集体。SDS聚丙烯酰胺凝胶电泳分析BSA聚集体证明,BSA聚集体的主要结合涉及分子间二硫键结合,并且用半胱氨酸封闭BSA分子中的游离巯基会导致超滤过程中BSA聚集体的数量显著减少。我们得出结论,超滤过程中BSA聚集的主要因素之一是通过半胱氨酸残基进行的二硫键分子间交换。我们还发现,BSA聚集导致α-螺旋从66%减少到50%,β-折叠从20%增加到36%,这可能是因为与分子间二硫键相关的半胱氨酸残基位于α-螺旋中。

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