首页> 外文期刊>Electronic Journal of Biotechnology >Rapid automated selection of mammalian cell line secreting high level of humanized monoclonal antibody using Clone Pix FL system and the correlation between exterior median intensity and antibody productivity
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Rapid automated selection of mammalian cell line secreting high level of humanized monoclonal antibody using Clone Pix FL system and the correlation between exterior median intensity and antibody productivity

机译:使用Clone Pix FL系统快速自动选择分泌高水平人源化单克隆抗体的哺乳动物细胞系,以及外部中值强度与抗体生产率之间的相关性

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The selection of high-producing mammalian cell lines is a crucial step in process development for the production of biopharmaceuticals. Previously, cloning by limiting dilution method was used to isolate monoclonal NS0 cells secreting high levels of humanized-C2 monoclonal antibodies. However limiting dilution method is time consuming, has low probability of monoclonality and is significantly limited by the number of clones that can be feasibly screened. In order to minimize the duration and to increase the probability of obtaining high-producing clones with high monoclonality, an automated colony picker, Clone Pix FL system was used to replace limiting dilution method. We were able to screen 1 x 105 clones secreting humanized monoclonal antibodies and high producer clones were selected in just 7 days. Briefly, semi-solid media was used to immobilize single cells separately and allow them to proliferate into discrete clones. The high viscosity nature of the semi-solid media retains the secreted products in the vicinity of the associated clones. Using Clone Pix FL system, all clones were screened and the producer clones with different exterior fluorescent intensities were automatically isolated. We were able to isolate rare high-producers (> 3000 FU) with frequency of as low as 0.003% of the population. A quantitative ELISA was also performed to evaluate the correlation between the fluorescence intensity of clones with its corresponding antibody productivity. Clones with fluorescence intensity of < 1000 FU showed relatively low antibody productivity compared with those greater than 1000 FU; however above this there was no correlation of production with the increase in fluorescence intensity. Hence, although the high-throughput, rapid and automated nature of Clone Pix FL system allows the screening of large number of cells in a short period of time with also an increased in the probability of obtaining rare and precious high-producing clones, downstream analysis are still vital to determine the ‘actual' and stable high producer clones.
机译:高产哺乳动物细胞系的选择是生物药物生产过程开发中的关键步骤。以前,通过有限稀释法克隆可用于分离分泌高水平人源化C2单克隆抗体的单克隆NS0细胞。然而,有限的稀释方法是费时的,具有低的单克隆可能性,并且受到可筛选的克隆数目的明显限制。为了最小化持续时间并增加获得具有高单克隆性的高产克隆的可能性,使用了自动菌落选择器Clone Pix FL系统来代替有限稀释法。我们能够筛选出1 x 105个分泌人源化单克隆抗体的克隆,并在短短7天内选择了高产量克隆。简而言之,使用半固体培养基分别固定单个细胞,并使它们增殖为离散的克隆。半固体培养基的高粘度性质将分泌产物保留在相关克隆附近。使用Clone Pix FL系统筛选所有克隆,并自动分离具有不同外部荧光强度的生产者克隆。我们能够分离出频率低至总人口0.003%的稀有高产菌(> 3000 FU)。还进行了定量ELISA,以评估克隆的荧光强度与其相应抗体生产率之间的相关性。荧光强度<1000 FU的克隆与大于1000 FU的克隆相比,抗体生产率相对较低;然而,在此之上,产量与荧光强度的增加没有相关性。因此,尽管Clone Pix FL系统具有高通量,快速和自动化的特性,可以在短时间内筛选大量细胞,但获得稀有和珍贵的高产克隆的可能性也有所增加,但下游分析对于确定“实际的”和稳定的高产克隆仍然至关重要。

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