拥挤环境中d-葡萄糖/d-半乳糖结合蛋白的结构和构象性质

A. Fonin, S. Silonov, Asiya K. Sitdikova, I. Kuznetsova, V. Uversky, K. Turoverov
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引用次数: 10

摘要

在聚乙二醇(PEG-12000、PEG-4000和PEG-600)、Ficoll-70和Dextran-70的浓溶液模拟的分子拥挤条件下,研究了d-葡萄糖/d-半乳糖结合蛋白(GGBP)的构象变化,它们的加入引起了GGBP分子的明显结构变化。所有peg都促进了GGBP的压实,并导致其结构的有序性增加。PEG-12000和PEG-4000的浓溶液引起GGBP聚集。虽然Ficoll-70和Dextran-70也促进了GGBP排序的增加,但不同人群的结构输出不同。例如,与缓冲液中的GGBP相比,该蛋白在peg存在时,其固有荧光光谱向短波区移动,而在Ficoll-70和Dextran-70存在时,其固有荧光光谱发生红移。据推测,这种差异可能是由于GGBP与糖基聚合物(Ficoll-70和Dextran-70)的特定相互作用,表明蛋白质在含有不同化学性质的分子聚合剂的溶液中可以采用不同的构象。研究还表明,所有被测试的拥挤剂都能够稳定GGBP的结构,使GGBP胍盐酸盐(GdnHCl)诱导的展开曲线向更高的变性剂浓度移动,但它们的稳定能力并不取决于聚合物分子的水动力尺寸。在所有测试的拥挤剂溶液中,GGBP的再折叠都因蛋白质聚集而复杂化。在PEG-12000的高浓度溶液中,再折叠蛋白的产率最低。这些数据支持了先前的观点,即大分子挤压剂对蛋白质的影响是一种相当复杂的现象,超出了排除的体积效应。
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Structure and Conformational Properties of d-Glucose/d-Galactose-Binding Protein in Crowded Milieu
Conformational changes of d-glucose/d-galactose-binding protein (GGBP) were studied under molecular crowding conditions modeled by concentrated solutions of polyethylene glycols (PEG-12000, PEG-4000, and PEG-600), Ficoll-70, and Dextran-70, addition of which induced noticeable structural changes in the GGBP molecule. All PEGs promoted compaction of GGBP and lead to the increase in ordering of its structure. Concentrated solutions of PEG-12000 and PEG-4000 caused GGBP aggregation. Although Ficoll-70 and Dextran-70 also promoted increase in the GGBP ordering, the structural outputs were different for different crowders. For example, in comparison with the GGBP in buffer, the intrinsic fluorescence spectrum of this protein was shifted to short-wave region in the presence of PEGs but was red-shifted in the presence of Ficoll-70 and Dextran-70. It was hypothesized that this difference could be due to the specific interaction of GGBP with the sugar-based polymers (Ficoll-70 and Dextran-70), indicating that protein can adopt different conformations in solutions containing molecular crowders of different chemical nature. It was also shown that all tested crowding agents were able to stabilize GGBP structure shifting the GGBP guanidine hydrochloride (GdnHCl)-induced unfolding curves to higher denaturant concentrations, but their stabilization capabilities did not depend on the hydrodynamic dimensions of the polymers molecules. Refolding of GGBP was complicated by protein aggregation in all tested solutions of crowding agents. The lowest yield of refolded protein was achieved in the highly concentrated solutions of PEG-12000. These data support the previous notion that the influence of macromolecular crowders on proteins is rather complex phenomenon that extends beyond the excluded volume effects.
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