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高效弱阳离子交换色谱法对脲还原变性溶菌酶的折叠研究
引用本文:刘红妮,王彦,龚波林,耿信笃.高效弱阳离子交换色谱法对脲还原变性溶菌酶的折叠研究[J].化学学报,2005,63(7):597-602.
作者姓名:刘红妮  王彦  龚波林  耿信笃
作者单位:(西北大学现代分离科学研究所 分离科学陕西省重点实验室 西安 710069)
基金项目:国家自然科学基金(No.20175016)资助项目
摘    要:用高效弱阳离子交换色谱(HPWCX)对脲还原变性溶菌酶(Lys)进行了复性研究. 在流动相中脲浓度固定为4.0 mol•L-1和选用对天然态蛋白有稳定作用的硫酸铵为盐或置换剂时, 在蛋白浓度为15.0~50.0 mg•mL-1时, HPWCX法比稀释法活性回收率高. 为了提高Lys的质量及活性回收率对所用色谱条件进行了优化研究, 当蛋白起始浓度为20.0 mg•mL-1时, Lys的质量回收率和活性收率分别为97.8%和95.4%. 表明此种方法简便且有可能对其他还原变性蛋白的复性具有通用性.

关 键 词:液相色谱  弱阳离子交换色谱  蛋白复性  溶菌酶  二硫键  
收稿时间:2004-3-12
修稿时间:2004-12-8

Study on Refolding of Urea-Reduced/Denatured Lysozyme by High-Performance Weak-cation Exchange Chromatography
LIU Hong-Ni,WANG Yan,GONG Bo-Lin,GENG Xin-Du.Study on Refolding of Urea-Reduced/Denatured Lysozyme by High-Performance Weak-cation Exchange Chromatography[J].Acta Chimica Sinica,2005,63(7):597-602.
Authors:LIU Hong-Ni  WANG Yan  GONG Bo-Lin  GENG Xin-Du
Institution:(Institute of Modern Separation Science, Key Laboratory of Modern Separation Science of Shaanxi Province, Xi'an 710069)
Abstract:The refolding of the urea-reduced/denatured lysozyme (Lys) by high-performance weak cation exchange chromatography was reported in this paper. With the presence of a fixed concentration of urea of 4.0 mol•L-1 and ammonium sulphate as salt or displacer having the stabilizing role to the structure of native protein molecules in the mobile phase employed, and when the Lys concentration was 15.0~50.0 mg•mL-1, the bioactivity recovery by the presented method was higher than that by usual dilution method. The optimization of chromatographic conditions for obtaining the high recoveries of both mass and bioactivity of Lys was investigated in detail. The recoveries of both mass and bioactivity could be raised up to 97.8% and 95.4% respectively, as the Lys concentration in sample solution was 20.0 mg•mL-1. The advantages of the presented method are simple operation, and high recoveries of both mass and bioactivity of Lys refolding, and thus it may possibly become a common method for many kinds of proteins.
Keywords:liquid chromatography  weak-cation exchange chromatography  protein refolding  lysozyme  disulfide bond
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