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High-level production of recombinant proteins in CHO cells using a dicistronic DHFR intron expression vector.

机译:使用双顺反子DHFR内含子表达载体在CHO细胞中大量生产重组蛋白。

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摘要

We have constructed expression vectors for Chinese hamster ovary (CHO) cells that produce both selectable marker and recombinant cDNA from a single primary transcript via differential splicing. These vectors produce stable CHO cell clones that, when pooled, produce abundant amounts of secreted recombinant proteins compared with the amounts produced by conventional expression approaches that have selectable marker and the cDNA of interest under control of separate transcription units. Our vectors divert most of the transcript to product expression while linking it, at a fixed ratio, to dihydrofolate reductase (DHFR) expression to allow selection of stable transfectants. Pools of clones with increased expression of the product gene can be efficiently generated by selection in methotrexate. The high level of expression from pools allows convenient and rapid production of milligram amounts of recombinant proteins.
机译:我们已经构建了中国仓鼠卵巢(CHO)细胞的表达载体,可以通过差异剪接从单个初级转录物中产生选择标记和重组cDNA。这些载体产生稳定的CHO细胞克隆,与合并的传统表达方法产生的数量相比,稳定的CHO细胞克隆在收集时会产生大量的重组蛋白,而传统的表达方法具有在单独的转录单位控制下的目标标记和选择性cDNA。我们的载体将大多数转录物转移至产物表达,同时将其以固定比例连接至二氢叶酸还原酶(DHFR)表达,以选择稳定的转染子。通过在甲氨蝶呤中进行选择可以有效地产生产物基因表达增加的克隆库。来自库的高水平表达允许方便且快速地产生毫克量的重组蛋白。

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