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High-level expression of recombinant IgG in the human cell line PER.C6

机译:重组IgG在人细胞系PER.C6中的高表达

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The number of therapeutic monoclonal antibodies in production is expected to rise rapidly in the next few years. As a result, there is much focus on the optimization of antibody expression platforms. Several issues are important including the speed of transition from bench to manufacturing, yield of IgG, and quality (particularly of the glycan structures present on immunoglobulins). We have characterized the human cell line PER.C6 for its ability to produce recombinant IgG. Production yields are still being optimized, but in nonfed batch culture, PER.C6 is able to grow to a cell density of 5x10(6) cells/mL and produce 300-500 mg/L IgG; this is likely to increase significantly in fed batch cultures. The generation of antibody-producing cell lines is fast, as rounds of amplification of inserted genes are not required for high production yields. The gene copy number of inserted genes is in the region of 1-10 copies per genome. In addition, PER.C6 is a human cell line, and so does not add glycans, which are immunogenic in humans. A core fucose molecule is essentially always present, and galactose residues are present at a physiological level (0, 1, and 2 galactose residues per glycan are present at a ratio of 1:2:1). No hybrid or high-mannose structures are seen.
机译:预计在未来几年中,生产中的治疗性单克隆抗体的数量将迅速增加。结果,非常关注抗体表达平台的优化。几个问题很重要,包括从实验台到生产的过渡速度,IgG的产率和质量(特别是免疫球蛋白上存在的聚糖结构)。我们已经表征了人类细胞系PER.C6产生重组IgG的能力。产量仍在优化中,但是在非分批培养中,PER.C6能够生长到5x10(6)个细胞/ mL的细胞密度,并产生300-500 mg / L IgG;在补料分批培养中,这可能会显着增加。产生抗体的细胞系的产生很快,因为不需要插入轮次的扩增基因即可获得高产量。每个基因组插入的基因的基因拷贝数在1-10个拷贝的范围内。此外,PER.C6是人类细胞系,因此不会添加在人类中具有免疫原性的聚糖。核心岩藻糖分子基本上总是存在,并且半乳糖残基以生理水平存在(每个聚糖中的0、1和2个半乳糖残基以1:2:1的比例存在)。没有看到杂合或高甘露糖结构。

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