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A multi-landing pad DNA integration platform for mammalian cell engineering

机译:用于哺乳动物细胞工程的多着陆垫DNA整合平台

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摘要

Engineering mammalian cell lines that stably express many transgenes requires the precise insertion of large amounts of heterologous DNA into well-characterized genomic loci, but current methods are limited. To facilitate reliable large-scale engineering of CHO cells, we identified 21 novel genomic sites that supported stable long-term expression of transgenes, and then constructed cell lines containing one, two or three ‘landing pad’ recombination sites at selected loci. By using a highly efficient BxB1 recombinase along with different selection markers at each site, we directed recombinase-mediated insertion of heterologous DNA to selected sites, including targeting all three with a single transfection. We used this method to controllably integrate up to nine copies of a monoclonal antibody, representing about 100 kb of heterologous DNA in 21 transcriptional units. Because the integration was targeted to pre-validated loci, recombinant protein expression remained stable for weeks and additional copies of the antibody cassette in the integrated payload resulted in a linear increase in antibody expression. Overall, this multi-copy site-specific integration platform allows for controllable and reproducible insertion of large amounts of DNA into stable genomic sites, which has broad applications for mammalian synthetic biology, recombinant protein production and biomanufacturing.
机译:稳定表达许多转基因的工程哺乳动物细胞系需要将大量的异源DNA精确插入到特征明确的基因组位点中,但是目前的方法受到限制。为了促进CHO细胞的可靠大规模工程化,我们鉴定了21个支持稳定长期表达转基因的新基因组位点,然后在选定的基因座处构建了包含一个,两个或三个“着陆垫”重组位点的细胞系。通过在每个位点使用高效的BxB1重组酶以及不同的选择标记,我们将重组酶介导的异源DNA插入到选定的位点,包括通过单个转染靶向全部三个。我们使用这种方法可控地整合多达九个拷贝的单克隆抗体,代表21个转录单位中约100 kb的异源DNA。由于整合的目标是预先验证的基因座,重组蛋白的表达在数周内保持稳定,整合的有效负载中抗体盒的其他拷贝导致抗体表达的线性增加。总体而言,该多拷贝位点特异性整合平台可将大量DNA进行可控制和可重现的插入稳定的基因组位点,在哺乳动物合成生物学,重组蛋白生产和生物制造中具有广泛的应用。

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