Column chromatographic separation characteristics of gene recombinant protein AxCeSD with N- and C-terminal histidine-tags

被引:0
|
作者
Hu, Songqing [1 ]
Shen, Xing [1 ]
Chen, Ping [1 ]
Yao, Min [2 ]
Hou, Yi [1 ]
Gao, Yonggui [2 ]
Isao, Tanaka [2 ]
Li, Lin [1 ]
机构
[1] School of Light Industry and Food Sciences, South China University of Technology, Guangdong Guangzhou 510640, China
[2] Faculty of Advanced Life Science, Hokkaido University, Sapporo 060-0810, Japan
来源
Huagong Xuebao/CIESC Journal | 2010年 / 61卷 / 01期
关键词
Affinity chromatography - Column chromatography - Hydrogen bonds - Purification - Biosynthesis - Liquid chromatography - Amino acids - Separation - Genes;
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学科分类号
摘要
Immobilization metal affinity chromatography (IMAC) and size-exclusive chromatography (SEC) have been widely used in the purification of recombinant protein. In order to apply the column chromatography to the separation and purification of the gene recombinant with histidine-tags, the column chromatographic separation characteristics of N-terminal histidine-tagged (N-AxCeSD) and C-terminal histidine-tagged (C-AxCeSD) gene recombinant protein AxCeSD, one of the subunit involved in the cellulose synthesis in Acetobacter xylinum were studied. In the ring-shaped three-dimensional structure of AxCeSD, N-terminal histidine-tags were located in the inner of ring, while C-terminal histidine-tags were located in the outer. A higher imidazole concentration was necessary for eluting the C-AxCeSD from the IMAC column due to the C-terminal histidine-tags had stronger chelating interaction with the Ni2+ on the IMAC media. Moreover, the retention time for eluting C-AxCeSD from the same SEC gel column was shorter than that for N-AxCeSD, because the larger protein homolog was formed in the C-AxCeSD solution through the inter-molecular hydrogen bonds between the C-terminal histidine-tags. © All Rights Reserved.
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页码:99 / 103
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