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从大肠杆菌中折叠和纯化不溶性(包涵体)蛋白质

Folding and Purification of Insoluble (Inclusion Body) Proteins from Escherichia coli.

作者信息

Wingfield Paul T, Palmer Ira, Liang Shu-Mei

机构信息

Protein Expression Laboratory, NIAMD/NIH, Bethesda, Maryland.

Agricultural Biotechnology Research Center, Academia Sinica, Taipei, Taiwan.

出版信息

Curr Protoc Protein Sci. 2014 Nov 3;78:6.5.1-6.5.30. doi: 10.1002/0471140864.ps0605s78.

Abstract

Heterologous expression of recombinant proteins in E. coli often results in the formation of insoluble and inactive protein aggregates, commonly referred to as inclusion bodies. To obtain the native (i.e., correctly folded) and hence active form of the protein from such aggregates, four steps are usually followed: (1) the cells are lysed, (2) the cell wall and outer membrane components are removed, (3) the aggregates are solubilized (or extracted) with strong protein denaturants, and (4) the solubilized, denatured proteins are folded with concomitant oxidation of reduced cysteine residues into the correct disulfide bonds to obtain the native protein. This unit features three different approaches to the final step of protein folding and purification. In the first, guanidine·HCl is used as the denaturant, after which the solubilized protein is folded (before purification) in an "oxido-shuffling" buffer system to increase the rate of protein oxidation. In the second, acetic acid is used to solubilize the protein, which is then partially purified by gel filtration before folding; the protein is then folded and oxidized by simple dialysis against water. Thirdly, folding and purification of a fusion protein using metal-chelate affinity chromatography are described.

摘要

重组蛋白在大肠杆菌中的异源表达常常导致不溶性且无活性的蛋白聚集体形成,通常称为包涵体。为了从这些聚集体中获得天然(即正确折叠)且因此具有活性形式的蛋白,通常遵循四个步骤:(1)裂解细胞,(2)去除细胞壁和外膜成分,(3)用强蛋白变性剂溶解(或提取)聚集体,以及(4)将溶解的变性蛋白折叠,同时将还原的半胱氨酸残基氧化成正确的二硫键以获得天然蛋白。本单元介绍了三种不同的蛋白质折叠和纯化最后一步的方法。第一种方法中,使用盐酸胍作为变性剂,之后在“氧化重排”缓冲系统中(在纯化之前)折叠溶解的蛋白以提高蛋白氧化速率。第二种方法中,使用乙酸溶解蛋白,然后在折叠之前通过凝胶过滤进行部分纯化;然后通过简单的对水透析使蛋白折叠并氧化。第三种方法描述了使用金属螯合亲和色谱对融合蛋白进行折叠和纯化。

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