| 人IL35-IgG4(Fc)融合蛋白在CHO/DG44细胞中的稳定表达 |
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| 引用本文: | 唐静,高闻达,张青,张大为,陈洋,何波,刘全胜.人IL35-IgG4(Fc)融合蛋白在CHO/DG44细胞中的稳定表达[J].生物工程学报,2009,25(1):0109-0115. |
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| 作者姓名: | 唐静 高闻达 张青 张大为 陈洋 何波 刘全胜 |
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| 作者单位: | 1. 四川大学生命科学学院,医学细胞生物学教研室,成都,610041
2. 哈佛大学医学院,波士顿,02115,美国 |
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| 基金项目: | 国家自然科学基金项目(No. 30371307)资助。 |
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| 摘 要: | 本研究利用基因重组技术构建人IL35-IgG4(Fc)融合基因真核表达载体, 稳定转染CHO/DG44细胞并检测重组蛋白的表达。主要采用聚合酶链式反应(PCR)从脂多糖(Lipopolysaccharides, LPS)诱导的人髓性白血病细胞株KG-I cDNA文库中克隆EBI3和IL-12p35 cDNA, 重叠PCR法连接2个片段, 并克隆到IgG4(Fc)- pOptiVEC?-TOPO?载体上,对新构建的IL-35-IgG4 (Fc) pOptiVEC?-TOPO?真核表达载体并进行酶切、测序、PCR鉴定; 脂质体法转染CHO/DG44细胞; RT-PCR检测转染结果, 采用a-MEM-培养基筛选实验组细胞, 对筛选的阳性克隆细胞再进行氨甲喋呤(Methotrexate, MTX)的加压筛选, ProteinG-Agarose纯化阳性克隆培养上清, 免疫印迹检测目的蛋白表达。结果显示IL-35-IgG4 (Fc) pOptiVEC?-TOPO?表达载体稳定转染CHO/DG44细胞并获得阳性克隆; SDS-PAGE电泳得到一条与预期相对分子质量大小相符的蛋白条带; 该蛋白能与羊抗人IgG4抗体特异结合。本实验获得了能够稳定表达具有稳定结构的IL35-IgG4(Fc)融合蛋白的CHO/DG44细胞株。
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| 关 键 词: | IL-35-IgG4(Fc)融合蛋白 重叠PCR 稳定转染 CHO/DG44细胞 MTX诱导的基因扩增 |
| 收稿时间: | 2008/7/30 0:00:00 |
Expression of humane IL-35-IgG4 (Fc) fusion protein in CHO/DG44 cells |
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| Jing Tang,Wenda Gao,Qing Zhang,Dawei Zhang,Yang Chen,Bo He and Quansheng Liu.Expression of humane IL-35-IgG4 (Fc) fusion protein in CHO/DG44 cells[J].Chinese Journal of Biotechnology,2009,25(1):0109-0115. |
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| Authors: | Jing Tang Wenda Gao Qing Zhang Dawei Zhang Yang Chen Bo He and Quansheng Liu |
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| Institution: | College of Life Science, Sichuan University, Chengdu 610041, China;Harvard Medical School, Boston 02115, USA;College of Life Science, Sichuan University, Chengdu 610041, China;College of Life Science, Sichuan University, Chengdu 610041, China;College of Life Science, Sichuan University, Chengdu 610041, China;College of Life Science, Sichuan University, Chengdu 610041, China;College of Life Science, Sichuan University, Chengdu 610041, China |
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| Abstract: | We constructed the eukaryotic expression vector of human IL-35-IgG4 (Fc)-pOptiVEC?-TOPO? by gene recombination technique and expressed the fusion protein human IL-35-IgG4 (Fc) in CHO/DG44 cells. The two components of the newly discovered cytokine human IL-35, EBI3 and IL-12p35, were amplified by PCR from the cDNA library derived from the KG-I cells after LPS induction. The two PCR-amplified cDNA fragments of human IL-35 were linked by over-lapping PCR and then cloned into the IgG4 (Fc)-pOptiVEC?-TOPO? vector. The constructed plasmid with the recombinant cDNA IL-35-IgG4 (Fc) was verified by restriction enzyme digestion analysis, PCR and DNA sequencing. The verified plasmid with the recombinant cDNA was transfected into CHO/DG44 cells using Lipofectamine? 2000. The success of the transfection was examined and confirmed by RT-PCR. After selection in a-MEM (-) medium, the IL-35-Ig G4 (Fc) positive CHO/DG44 clones were chosen and the media from these positive clones were collected to be used to purify the fusion protein. The positive CHO/DG44 clones were further cultured in increasing concentrations of MTX and the expression levels of the fusion protein IL-35-Ig G4 (Fc) were repetitively induced by MTX-induced gene amplification. The IL-35-Ig G4 (Fc) fusion protein was purified from the media collected from the positive CHO/DG44 clones by protein G affinity chromatography and then identified by SDS-PAGE and Western blotting. The results showed that one protein band was found to match well with the predicted relative molecular mass of human IL-35-IgG4 (Fc) and this protein could specifically bind to anti-human IgG4 (Fc) monoclonal antibody. In conclusion, our study successfully established an IL-35-IgG4 (Fc) positive DG44 cell line which could stably express IL-35-IgG4 (Fc) fusion protein. |
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| Keywords: | IL-35-IgG4 (Fc) fusion protein over-lapping PCR stable transfection CHO/DG44cell lines MTX-induced gene amplification |
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