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首页> 外文期刊>Journal of Biotechnology >Identification of cellular genes critical to recombinant protein production using a Gaussia luciferase-based siRNA screening system
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Identification of cellular genes critical to recombinant protein production using a Gaussia luciferase-based siRNA screening system

机译:使用基于高斯荧光素酶的siRNA筛选系统鉴定对重组蛋白生产至关重要的细胞基因

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Development of high-throughput functional genomic screening, including siRNA screening, provides a novel approach for quick identification of critical factors involved in biological processes. Here, we apply this strategy to search for cellular genes involved in recombinant protein production. Since most of biopharmaceutical proteins are secreted proteins, we develop a cell-based reporter assay using a secreted luciferase, Gaussia luciferase (Gluc), as the reporter. Human embryonic kidney 293 (HEK293) cells transiently transfected with the Gluc reporter plasmid are used to screen our siRNA panel. Three cellular genes, CCAAT/enhancer binding protein gamma (CEBPG), potassium channel tetramerisation domain containing 2 (KCTD2), transmembrane protein 183A (TMEM183A), were isolated from the screening. Production of erythropoietin (EPO) was significantly inhibited when CEBPG, KCTD2, and TMEM183A were knocked down. Furthermore, overexpression of CEBPG is shown to significantly improve production of recombinant EPO, interferon d, and monoclonal antibody in HEK293 and Chinese hamster ovary cells. Collectively, this novel Gluc-based siRNA screening system is proven to be a useful tool for investigation of secreted protein production in mammalian cells.
机译:高通量功能基因组筛选(包括siRNA筛选)的开发提供了一种新颖的方法,可以快速识别生物过程中涉及的关键因素。在这里,我们应用这种策略来搜索参与重组蛋白生产的细胞基因。由于大多数生物制药蛋白都是分泌蛋白,因此我们使用分泌的荧光素酶Gaussia luciferase(Gluc)作为报道分子,开发了基于细胞的报道分子测定法。用Gluc报告质粒瞬时转染的人胚肾293(HEK293)细胞用于筛选siRNA。从筛选中分离出三个细胞基因,CCAAT /增强子结合蛋白γ(CEBPG),含2个钾通道四聚体结构域(KCTD2),跨膜蛋白183A(TMEM183A)。当敲除CEBPG,KCTD2和TMEM183A时,促红细胞生成素(EPO)的产生被显着抑制。此外,CEBPG的过表达可显着改善HEK293和中国仓鼠卵巢细胞中重组EPO,干扰素d和单克隆抗体的产生。总的来说,这种新颖的基于Gluc的siRNA筛选系统被证明是研究哺乳动物细胞中分泌的蛋白质生产的有用工具。

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