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蛋白质变性对溶菌酶溶液中聚集和胶凝的影响。

Effects of Protein Unfolding on Aggregation and Gelation in Lysozyme Solutions.

机构信息

Department of Chemical and Biomolecular Engineering, University of Maryland, College Park, MD 20742, USA.

Institute for Physical Science and Technology, University of Maryland, College Park, MD 20742, USA.

出版信息

Biomolecules. 2020 Sep 2;10(9):1262. doi: 10.3390/biom10091262.

Abstract

In this work, we investigate the role of folding/unfolding equilibrium in protein aggregation and formation of a gel network. Near the neutral pH and at a low buffer ionic strength, the formation of the gel network around unfolding conditions prevents investigations of protein aggregation. In this study, by deploying the fact that in lysozyme solutions the time of folding/unfolding is much shorter than the characteristic time of gelation, we have prevented gelation by rapidly heating the solution up to the unfolding temperature (80 °C) for a short time (30 min.) followed by fast cooling to the room temperature. Dynamic light scattering measurements show that if the gelation is prevented, nanosized irreversible aggregates (about 10-15 nm radius) form over a time scale of 10 days. These small aggregates persist and aggregate further into larger aggregates over several weeks. If gelation is not prevented, the nanosized aggregates become the building blocks for the gel network and define its mesh length scale. These results support our previously published conclusion on the nature of mesoscopic aggregates commonly observed in solutions of lysozyme, namely that aggregates do not form from lysozyme monomers in their native folded state. Only with the emergence of a small fraction of unfolded proteins molecules will the aggregates start to appear and grow.

摘要

在这项工作中,我们研究了折叠/去折叠平衡在蛋白质聚集和凝胶网络形成中的作用。在接近中性 pH 值和低缓冲离子强度的条件下,在展开条件下形成的凝胶网络会阻碍对蛋白质聚集的研究。在这项研究中,通过利用这样一个事实,即在溶菌酶溶液中,折叠/去折叠的时间比凝胶化的特征时间短得多,我们通过快速将溶液加热到展开温度(80°C)来防止凝胶化,时间很短(30 分钟),然后快速冷却到室温。动态光散射测量表明,如果防止凝胶化,纳米级不可逆转的聚集体(约 10-15nm 半径)会在 10 天的时间尺度内形成。这些小聚集体会持续存在,并在数周内进一步聚集形成更大的聚集体。如果不防止凝胶化,纳米级聚集体就会成为凝胶网络的构建块,并定义其网格长度尺度。这些结果支持了我们之前关于溶菌酶溶液中常见的介观聚集体的本质的结论,即聚集体不是从天然折叠状态的溶菌酶单体中形成的。只有当一小部分去折叠的蛋白质分子出现时,聚集体才会开始出现并生长。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/61b0/7563771/9ac15238eab0/biomolecules-10-01262-g001.jpg

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