重组人粒细胞-巨噬细胞集落刺激因子(9-127)/白细胞介素-6(29-184)融合蛋白在大肠杆菌中的高效表达与纯化
High-level expression and purification of recombinant huGM-CSF (9-127)/IL-6 (29-184) fusion protein in Escherichia coil.
作者信息
Sun Qiang-ming, Jiang Hong-chao, Xu Wei-ming, Liu Xin, Dai Chang-bai, Sun Mao-sheng
机构信息
Department of Molecular Biology, Institute of Medical Biology, Chinese Academy of Medical Sciences and Peking Union Medical College, Kunming, Yunnan 650118, PR China.
出版信息
Protein Expr Purif. 2005 Aug;42(2):278-85. doi: 10.1016/j.pep.2005.04.007.
As HuGM-CSF and huIL-6 seem to have synergistic and complementary actions, researchers have proposed that fusion proteins incorporating these two cytokines could show increased biological activity, especially in terms of hematopoietic function. Here, we sought to obtain a functional GM-CSF/IL-6 fusion protein and to investigate its biological activities in vitro. A novel construct encoding a fusion protein of huGM-CSF (9-127) and IL-6 (29-184) was generated in the pBV220 expression vector by step-by-step cloning. Amino acids 1-8 of huGM-CSF and amino acids 1-28 of huIL-6 were deleted by PCR. The mutant huGM-CSF (9-127) and huIL-6 (29-184) cDNAs were linked via a linker sequence encoding 15 amino acid residues (G-G-S-G-S)3. Direct sequencing was used to confirm the validity of the desired construct, and the fusion protein was expressed in Escherichia coli host strain BL21 (DE3) in the form of inclusion bodies (IBs). The expression level was more than 25% of the total cell lysate, and a novel purification and refolding strategy was used to isolate the fusion protein product. Inclusion bodies were purified by Q Sepharose H.P. ion exchange in 8 mol/L urea, followed by in situ refolding by Sephacryl S-200. The renatured fusion proteins were obtained at a purity of >95%, and the strategy of refolding on the gel filtration column was found to be efficient, with a relative refolding rate of 80%. This entire refolding and purification procedure could be performed within one day and may prove applicable to large-scale purification and refolding of recombinant proteins from IBs in E. coli. This new method was used to obtain huGM-CSF (9-127)/IL-6 (29-184) fusion protein with high purity and biological activity. MTT assays in TF-1 and B9 cell lines showed that the specific biological activity of huGM-CSF was 1.14+/-0.10 x 10(8) U/mg, and that for huIL-6 was 1.89+/-0.11 x 10(7) U/mg. The fusion protein exhibited enhanced huGM-CSF, but similar huIL-6 biological activities compared with those of either GM-CSF or IL-6 alone. This suggests that our novel huGM-CSF (9-127)/IL-6 (29-184) fusion protein may hold future promise as a therapeutic agent.
由于人粒细胞巨噬细胞集落刺激因子(HuGM-CSF)和人白细胞介素-6(huIL-6)似乎具有协同和互补作用,研究人员提出,包含这两种细胞因子的融合蛋白可能具有更高的生物活性,特别是在造血功能方面。在此,我们试图获得一种功能性GM-CSF/IL-6融合蛋白,并在体外研究其生物活性。通过逐步克隆,在pBV220表达载体中构建了一种编码huGM-CSF(9-127)和IL-6(29-184)融合蛋白的新型构建体。通过PCR删除了huGM-CSF的1-8位氨基酸和huIL-6的1-28位氨基酸。突变型huGM-CSF(9-127)和huIL-6(29-184)的cDNA通过编码15个氨基酸残基(G-G-S-G-S)3的接头序列连接。直接测序用于确认所需构建体的有效性,融合蛋白以包涵体(IBs)的形式在大肠杆菌宿主菌株BL21(DE3)中表达。表达水平超过总细胞裂解物的25%,并采用一种新型的纯化和复性策略来分离融合蛋白产物。包涵体在8 mol/L尿素中通过Q Sepharose H.P.离子交换进行纯化,然后通过Sephacryl S-200进行原位复性。复性后的融合蛋白纯度>95%,发现凝胶过滤柱上的复性策略是有效的,相对复性率为80%。整个复性和纯化过程可在一天内完成,可能适用于从大肠杆菌包涵体中大规模纯化和复性重组蛋白。这种新方法用于获得具有高纯度和生物活性的huGM-CSF(9-127)/IL-6(29-184)融合蛋白。在TF-1和B9细胞系中的MTT分析表明,huGM-CSF的比生物活性为1.14±0.10×10(8) U/mg,huIL-6的比生物活性为1.89±0.11×10(7) U/mg。与单独的GM-CSF或IL-6相比,融合蛋白表现出增强的huGM-CSF活性,但huIL-6生物活性相似。这表明我们新型的huGM-CSF(9-127)/IL-6(29-184)融合蛋白可能作为一种治疗剂具有未来应用前景。
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