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Transient expression of human antibodies in mammalian cells

机译:哺乳动物细胞中人抗体的瞬时表达

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Recombinant expression of antibody molecules in mammalian cells offers important advantages over traditionally utilized bacterial expression, including glycosylation required for antibody functionality and markedly reduced levels of endotoxin contamination. Advances in transient mammalian expression systems enable high yields ( 100 mg/liter) that now allow for effective recombinant antibody production at a reasonable cost. Here, we provide step-by-step protocols for the design and recombinant expression of full-length IgG antibodies and antibody-derived constructs (including Fab, Fc-fusions and bispecifics) in mammalian cells. Antibody constructs are designed by combining antibody variable domains, generated by phage display or derived from human/humanized monoclonals, with constant regions. The constructs are then expressed from mammalian vectors, secreted into culture media, purified by affinity chromatography and characterized by biolayer interferometry. This article provides detailed protocols, sequences and strategies that allow the expression and purification of endotoxin-free antibody reagents suitable for testing in animal models within a 3-week time frame.
机译:哺乳动物细胞中抗体分子的重组表达具有超过传统使用的细菌表达的重要优势,包括抗体功能所需的糖基化并显着降低内毒素污染水平。瞬时哺乳动物表达系统的进展使得能够以合理的成本允许有效的重组抗体产生的高产率(& 100 mg /升)。在这里,我们为哺乳动物细胞中的全长IgG抗体和抗体衍生的构建体(包括Fab,Fc-Fusions和Bispecifics)的设计和重组表达提供逐步方案。抗体构建体通过组合抗体可变结构域,由噬菌体显示器产生或衍生自人/人源化单烯烃,具有恒定的区域。然后将构建体从分泌到培养基中的哺乳动物载体中,通过亲和层析纯化,并通过Biolayer干涉测定法。本文提供了详细的方案,序列和策略,其允许在3周的时间框架内的用于在动物模型中测试的内毒素的无抗体试剂的表达和纯化。

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