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Production of stable bispecific IgG1 by controlled Fab-arm exchange

机译:通过受控Fab臂交换产生稳定的双特异性IgG1

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摘要

The manufacturing of bispecific antibodies can be challenging for a variety of reasons. For example, protein expression problems, stability issues, or the use of non-standard approaches for manufacturing can result in poor yield or poor facility fit. In this paper, we demonstrate the use of standard antibody platforms for large-scale manufacturing of bispecific IgG1 by controlled Fab-arm exchange. Two parental antibodies that each contain a single matched point mutation in the CH3 region were separately expressed in Chinese hamster ovary cells and manufactured at 1000 L scale using a platform fed-batch and purification process that was designed for standard antibody production. The bispecific antibody was generated by mixing the two parental molecules under controlled reducing conditions, resulting in efficient Fab-arm exchange of >95% at kg scale. The reductant was removed via diafiltration, resulting in spontaneous reoxidation of interchain disulfide bonds. Aside from the bispecific nature of the molecule, extensive characterization demonstrated that the IgG1 structural integrity was maintained, including function and stability. These results demonstrate the suitability of this bispecific IgG1 format for commercial-scale manufacturing using standard antibody manufacturing techniques.
机译:由于各种原因,双特异性抗体的生产可能具有挑战性。例如,蛋白质表达问题,稳定性问题或使用非标准方法进行生产都可能导致不良的产量或不良的设备适应性。在本文中,我们证明了通过可控Fab臂交换大规模生产双特异性IgG1的标准抗体平台的使用。在中国仓鼠卵巢细胞中分别表达两种各自在CH3区域中包含单个匹配点突变的亲本抗体,并使用平台进料分批和纯化工艺(设计用于标准抗体生产)以1000 L规模生产。通过在受控的还原条件下将两个亲本分子混合来生成双特异性抗体,从而导致有效的Fab臂交换(公斤级)> 95%。通过渗滤除去还原剂,导致链间二硫键自发再氧化。除了分子的双特异性性质之外,广泛的表征表明,IgG1的结构完整性得以保持,包括功能和稳定性。这些结果证明了这种双特异性IgG1格式适用于使用标准抗体生产技术进行商业规模生产。

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