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Renaturation of recombinant human granulocyte colony-stimulating factor produced from Escherichia coli using size exclusion chromatography

机译:使用大小排阻色谱法对大肠杆菌产生的重组人粒细胞集落刺激因子进行复性

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Refolding with simultaneously partial purification of recombinant human granulocyte colony-stimulating factor (rhG-CSF) expressed in Escherichia coli (E. coli) by size exclusion chromatography (SEC) is presented in this work. The solution containing the denatured and reduced rhG-CSF in 8.0 mol(.) L-1 urea extracted from the inclusion body was directly injected into a Superdex 75 column and the refolded rhG-CSF was obtained after elution from the column. Several factors, including the concentration of urea in the mobile phase, pH, flow rate, concentration of glutathione, and ratio of GSH to GSSG, concentration of glycerol, sample loading volume, effecting the aim protein refolding were investigated in details. With the selected optimal conditions, the denatured and reduced rhG-CSF was successfully refolded by SEC, and was partially purified during the chromatographic process. When 200 mu L of denatured rhG-CSF at a concentration of 2.3 mg(.) mL(-1) was loaded on the SEC column, rhG-CSF with specific activity of 1.2 x 10(8) IU (.) mg(-1), purity of 83%, and mass recovery of 30% was obtained.
机译:通过大小排阻色谱法(SEC)进行重组并同时部分纯化在大肠杆菌(E. coli)中表达的重组人粒细胞集落刺激因子(rhG-CSF)。从包涵体中提取的在8.0 mol(。)L-1尿素中含有变性和还原的rhG-CSF的溶液直接注入Superdex 75色谱柱,并从色谱柱洗脱后获得重折叠的rhG-CSF。详细研究了流动相中尿素的浓度,pH,流速,谷胱甘肽的浓度以及GSH与GSSG的比例,甘油的浓度,样品上样量以及影响目标蛋白质复性的几个因素。在选定的最佳条件下,变性并还原的rhG-CSF通过SEC成功折叠,并在色谱过程中部分纯化。当将200μL变性的rhG-CSF以2.3 mg(。)mL(-1)的浓度加载到SEC柱上时,具有1.2 x 10(8)IU(。)mg(-)比活的rhG-CSF。 1)的纯度为83%,质量回收率为30%。

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