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首页> 外文期刊>Journal of Biotechnology >Proposal for a better integration of bacterial lysis into the production of plasmid DNA at large scale
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Proposal for a better integration of bacterial lysis into the production of plasmid DNA at large scale

机译:关于将细菌裂解更好地整合到质粒DNA生产中的建议

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The paper addresses the question of how to achieve bacterial lysis in large-scale plasmid DNA production processes, where conventional alkaline lysis may become awkward to handle. Bacteria were grown in shaker flasks and a bioreactor. Suboptimal growth conditions were found advantageous for stable plasmid production at high copy numbers (up to 25mg/L could be achieved). Cells were harvested by filtration in the presence of a filter aid. A linear relationship between the biomass and the optimal filter aid concentration in terms of back pressure could be established. Bacteria-containing filter cakes were washed with isotonic buffer and lysis was achieved in situ by a two-step protocol calling for fragilisation of the cells followed by heat lysis in a suitable buffer. RNA and other soluble cell components where washed out of the cake during this step, while the plasmid DNA was retained. Afterwards a clear lysate containing relatively pure plasmid DNA could be eluted from the cake mostly as the desired supercoiled topoisomer, while cell debris and genomic DNA were retained. Lysis is, thus, integrated not only with cell capture but also with a significant degree of isolation/purification, as most impurities were considerably reduced during the procedure.
机译:本文探讨了如何在大规模质粒DNA生产过程中实现细菌裂解的问题,而传统的碱性裂解方法可能难以处理。细菌在摇瓶和生物反应器中生长。发现亚最佳生长条件有利于在高拷贝数下稳定生产质粒(最高可达25mg / L)。在助滤剂存在下通过过滤收集细胞。可以建立生物质和最佳助滤剂浓度之间在背压方面的线性关系。用等渗缓冲液洗涤含细菌的滤饼,并通过两步方案原位裂解,该方案要求将细胞裂解,然后在合适的缓冲液中热裂解。在此步骤中,RNA和其他可溶性细胞成分从滤饼中洗出,而质粒DNA被保留。之后,含有相对纯质粒DNA的澄清裂解液可以从滤饼中洗脱出来,主要是所需的超螺旋拓扑异构体,而细胞碎片和基因组DNA却保留了下来。因此,裂解不仅与细胞捕获结合,而且与分离/纯化的程度也很高,因为在此过程中,大多数杂质都得到了大大减少。

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