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Inducible Escherichia coli fermentation for increased plasmid DNA production

机译:诱导型大肠杆菌发酵可提高质粒DNA的产量

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Bacterial plasmids are the vectors of choice for DNA vaccines and short-term gene therapeutics. Growing plasmid DNA by microbial (Escherichia coli) fermentation is usually combined with alkaline lysis/chromatography methods of purification. To date, typical plasmid fermentation media and processes result in yields of 100-250 mg of plasmid DNA/I of culture medium, using standard high-copy pUC origin-containing plasmids. In order to address this initial and yield-limiting upstream step, we identified novel fermentation control parameters for fed-batch fermentation. The resulting fermentation strategies significantly increased specific plasmid yield with respect to cell mass while enhancing plasmid integrity and maintaining supercoiled DNA content. Fed-batch fermentation yield exceeding 1000 mg of plasmid DNA/I was obtained after reduction of plasmid-mediated metabolic burden during growth, and yields up to 1500 mg of plasmid DNA/I have been achieved with optimized plasmid backbones. Interestingly, by inducing high plasmid levels after sufficient biomass accumulation at low temperature and restricted growth, cells were able to tolerate significantly higher plasmid quantities than cells grown by conventional processes. This S-10-fold increase in plasmid yield dramatically decreases plasmid manufacturing costs and improves the effectiveness of downstream purification by reducing the fraction of impurities.
机译:细菌质粒是DNA疫苗和短期基因治疗药物的选择载体。通过微生物(大肠杆菌)发酵生长的质粒DNA通常与碱性裂解/色谱法纯化结合使用。迄今为止,使用标准的高拷贝含pUC起点的质粒,典型的质粒发酵培养基和工艺可产生100-250 mg培养基的质粒DNA / I。为了解决此初始和限制产量的上游步骤,我们确定了补料分批发酵的新型发酵控制参数。相对于细胞质量,所得的发酵策略显着提高了特定质粒的产量,同时增强了质粒的完整性并保持了超螺旋DNA的含量。在生长过程中减少质粒介导的代谢负担后,补料分批发酵的产量超过了1000 mg质粒DNA / I,并且使用优化的质粒骨架获得了高达1500 mg质粒DNA / I的产量。有趣的是,通过在低温下足够的生物量积累和受限的生长后诱导高质粒水平,与常规方法生长的细胞相比,细胞能够耐受更高的质粒数量。质粒产量的这种S-10-倍增加大大降低了质粒的生产成本,并通过减少杂质的比例提高了下游纯化的效率。

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