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Effect of Production Method and Gene Amplification on the Glycosylation Pattern of a Secreted Reporter Protein in CHO Cells

机译:生产方法和基因扩增对CHO细胞分泌的报道蛋白糖基化模式的影响

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摘要

We have investigated the independent effects of selective gene amplification (using the dhfr amplifiable selection marker) and culture operating strategy (batch vs repeated fed-batch vs semicontinuous perfusion) on the glycosylation of a recombinant reporter protein (secreted alkaline phosphatase,SEAP) produced in transfected Chinese hamster ovary (CHO) cells.HPLC analyses coupled with susceptibility to various exoglycosidases were used to determine the N-glycosylation profile of SEAP samples.The dhfr amplified cell line yielded an almost 10-fold increase in specific productivity as compared to that of the unamplified cell line.The glycosylation pattern of the reporter protein produced in batch bioreactor cultures of the amplified cell line showed only slight differences as compared to the glycosylation pattern of the protein from batch bioreactor cultures of the unamplified cell line.In contrast,analysis of SEAP glycosylation structures from the protein isolated from semicontinuous perfusion cultures indicated that both relative glycan content and extent of sialylation were increased as compared to samples isolated from repeated fed-batch cultures.These results suggest that the slow growing perfusion cultures produce more completely glycosylated proteins than the faster growing repeated fed-batch cultures.
机译:我们研究了选择性基因扩增(使用dhfr可扩增选择标记)和培养操作策略(批处理vs重复进料批处理vs半连续灌注)对重组报导蛋白(分泌型碱性磷酸酶,SEAP)糖基化的独立影响。转染的中国仓鼠卵巢(CHO)细胞.HPLC分析和对各种外切糖苷酶的敏感性被用来确定SEAP样品的N-糖基化谱图。与未扩增细胞系的分批生物反应器培养物中的蛋白质的糖基化模式相比,在扩增细胞系的分批生物反应器培养物中产生的报告蛋白的糖基化模式仅显示出细微的差异。来自半连续PE的蛋白质的SEAP糖基化结构灌注培养表明,与从重复补料分批培养物中分离的样品相比,相对聚糖含量和唾液酸化程度都增加了。

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