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高浓度变性及变性/还原溶菌酶的复性

Refolding of denatured and denatured/reduced lysozyme at high concentrations.

作者信息

Raman B, Ramakrishna T, Rao C M

机构信息

Centre for Cellular and Molecular Biology, Hyderabad 500 007, India.

出版信息

J Biol Chem. 1996 Jul 19;271(29):17067-72. doi: 10.1074/jbc.271.29.17067.

DOI:10.1074/jbc.271.29.17067
PMID:8663382
Abstract

Refolding of proteins at high concentrations often results in aggregation. To gain insight into the molecular aspects of refolding and to improve the yield of active protein, we have studied the refolding of lysozyme either from its denatured state or from its denatured/reduced state. Refolding of denatured lysozyme, even at 1 mg/ml, yields fully active enzyme without aggregation. However, refolding of denatured/reduced lysozyme into buffer that lacks thiol/disulfide reagents leads to aggregation. Thiol/disulfide redox reagents such as cysteine/cystine and reduced/oxidized glutathione facilitate the renaturation, with the yield depending on their absolute concentrations. We have obtained an approximately 70% renaturation yield upon refolding of lysozyme at 150 microgram/ml. The cysteine/cystine redox system is more efficient compared with the glutathione redox system. When lysozyme is refolded in the absence of redox reagents, a transient intermediate that has regained a significant amount of secondary structure is formed. The tryptophans in this intermediate are as exposed to water as in the fully unfolded protein. It shows increased exposure of hydrophobic surfaces compared with the native or completely unfolded enzyme. This aggregation-prone intermediate folds to active enzyme upon addition of oxidized glutathione before the aggregation process starts. These properties of the intermediate in the refolding pathway of lysozyme are similar to those proposed for the molten globule.

摘要

高浓度蛋白质的重折叠常常导致聚集。为了深入了解重折叠的分子机制并提高活性蛋白的产量,我们研究了溶菌酶从变性状态或变性/还原状态的重折叠过程。即使在1mg/ml的浓度下,变性溶菌酶的重折叠也能产生无聚集的完全活性酶。然而,将变性/还原的溶菌酶重折叠到缺乏硫醇/二硫键试剂的缓冲液中会导致聚集。硫醇/二硫键氧化还原试剂,如半胱氨酸/胱氨酸和还原型/氧化型谷胱甘肽,有助于复性,产量取决于它们的绝对浓度。当溶菌酶在150微克/毫升的浓度下重折叠时,我们获得了大约70%的复性产量。与谷胱甘肽氧化还原系统相比,半胱氨酸/胱氨酸氧化还原系统更有效。当溶菌酶在没有氧化还原试剂的情况下重折叠时,会形成一种重新获得大量二级结构的瞬时中间体。该中间体中的色氨酸与完全未折叠的蛋白质一样暴露于水中。与天然或完全未折叠的酶相比,它显示出疏水表面的暴露增加。在聚集过程开始之前,加入氧化型谷胱甘肽后,这种易于聚集的中间体折叠成活性酶。溶菌酶重折叠途径中中间体的这些性质与熔球态所提出的性质相似。

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Refolding of denatured and denatured/reduced lysozyme at high concentrations.高浓度变性及变性/还原溶菌酶的复性
J Biol Chem. 1996 Jul 19;271(29):17067-72. doi: 10.1074/jbc.271.29.17067.
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