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Refolding of recombinant human interferon alpha-2a from Escherichia coli by urea gradient size exclusion chromatography

机译:尿素梯度大小排阻色谱法从大肠杆菌中重组重组人干扰素α-2a

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摘要

Protein refolding is still a puzzle in the production of recombinant proteins expressed as inclusion bodies (IBs) in Escherichia coli. Gradient size exclusion chromatography (SEC) is a recently developed method for refolding of recombinant proteins in IBs. In this study, we used a decreasing urea gradient SEC for the refolding of recombinant human interferon alpha-2a (rhIFN alpha-2a) which was overexpressed as IBs in E. coli. In chromatographic process, the denatured rhIFN alpha-2a would pass along the 8.0-3.0 M urea gradient and refold gradually. Several operating conditions, such as final concentration of urea along the column, gradient length, the ratio of reduced to oxidized glutathione and flow rate were investigated, respectively. Under the optimum conditions, 1.2 x 10(8) IU/mg of specific activity and 82% mass recovery were obtained from the loaded 10 ml of 1.75 mg/ml denatured protein, and rhIFN alpha-2a was also purified during this process with the purity of higher than 92%. Compared with dilution method, urea gradient SEC was more efficient for the rhIFN alpha-2a refolding in terms of specific activity and mass recovery.
机译:在大肠杆菌中表达为包涵体(IBs)的重组蛋白的生产中,蛋白复性仍然是一个难题。梯度大小排阻色谱法(SEC)是最近开发的用于重组蛋白在IBs中重折叠的方法。在这项研究中,我们使用了递减的尿素梯度SEC来重组重组人干扰素α-2a(rhIFN alpha-2a),而重组人干扰素α-2a在大肠杆菌中作为IBs过表达。在色谱过程中,变性的rhIFNα-2a将沿着8.0-3.0 M尿素梯度通过并逐渐重折叠。分别研究了几种操作条件,例如沿塔的最终尿素浓度,梯度长度,还原型与氧化型谷胱甘肽的比例以及流速。在最佳条件下,从装载的10 ml的1.75 mg / ml变性蛋白中获得1.2 x 10(8)IU / mg的比活和82%的质量回收率,并且在此过程中还使用rhIFNα-2a纯化了rhIFNα-2a。纯度高于92%。与稀释法相比,尿素梯度SEC在比活度和质量回收率方面对rhIFNα-2a重折叠更为有效。

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