应用 FISH 技术鉴定不同高表达重组 CHO 细胞系的转基因整合位点。
Identification of transgene integration loci of different highly expressing recombinant CHO cell lines by FISH.
机构信息
Austrian Center of Biopharmaceutical Technology, Muthgasse 18, 1190, Vienna, Austria,
出版信息
Cytotechnology. 2006 Jul;51(3):171-82. doi: 10.1007/s10616-006-9029-0. Epub 2006 Nov 15.
Abstract
Recombinant CHO cell lines have integrated the expression vectors in various parts of the genome leading to different levels of gene amplification, productivity and stability of protein expression. Identification of insertion sites where gene amplification is possible and the transcription rate is high may lead to systems of site-directed integration and will significantly reduce the process for the generation of stably and highly expressing recombinant cell lines. We have investigated a broad range of recombinant cell lines by FISH analysis and Giemsa-Trypsin banding and analysed their integration loci with regard to the extent of methotrexate pressure, transfection methods, promoters and protein productivities. To summarise, we found that the majority of our high producing recombinant CHO cell lines had integrated the expression construct on a larger chromosome of the genome. Furthermore, except from two cell lines, the exogene was integrated at a single site. The dhfr selection marker was co-localised to the target gene.
摘要
重组 CHO 细胞系已将表达载体整合到基因组的不同部位,从而导致基因扩增、蛋白质表达的产量和稳定性的不同。鉴定可能发生基因扩增且转录率较高的插入位点可能会导致定点整合系统的出现,并将大大缩短稳定且高效表达重组细胞系的生成过程。我们通过 FISH 分析和 Giemsa-Trypsin 带型分析研究了广泛的重组细胞系,并根据甲氨蝶呤压力、转染方法、启动子和蛋白质产量分析了它们的整合位点。总之,我们发现我们的大多数高产重组 CHO 细胞系已将表达构建体整合到基因组的较大染色体上。此外,除了两个细胞系之外,外源基因都整合到一个单一的位置。dhfr 选择标记与靶基因共定位。
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