Riesenberg D, Menzel K, Schulz V, Schumann K, Veith G, Zuber G, Knorre W A
Zentralinstitut für Mikrobiologie und experimentelle Therapie der AdW der DDR, Jena.
Appl Microbiol Biotechnol. 1990 Oct;34(1):77-82. doi: 10.1007/BF00170927.
A defined medium was developed which, by means of a specific fed-batch mode, allows growth of the recombinant Escherichia coli strain TG1 (pBB210) up to a cell density of 60 g dry weight/l. Apart from glucose and aqueous ammonia fed as carbon and nitrogen sources, it was necessary to supply other nutrients or O2-enriched air. Aqueous ammonia also served for pH control. The pO2 level was kept at 20% saturation via closed-loop controls operating the two output variables of stirrer speed and glucose feeding rate. This fed-batch method prevented significant accumulation of acetate and other metabolic by-products. The recombinant E. coli expressed interferon alpha 1 more efficiently at a lower specific growth rate (muPr approximately 0.15 h-1) than at the maximum specific growth rate (mu max = 0.45 h-1). Therefore, fermentation in the batch phase at mu max was only allowed to continue up to a medium cell density. In the succeeding fed-batch phase, the specific growth rate was reduced to muPr by increasing the stirrer speed according to an empirically developed time scale.
开发了一种特定培养基,通过特定的补料分批培养模式,可使重组大肠杆菌菌株TG1 (pBB210)生长至细胞密度达到60 g干重/升。除了以葡萄糖和氨水作为碳源和氮源进料外,还需要供应其他营养物质或富氧空气。氨水也用于pH控制。通过操作搅拌器速度和葡萄糖进料速率这两个输出变量的闭环控制,将pO2水平保持在20%饱和度。这种补料分批培养方法可防止乙酸盐和其他代谢副产物的大量积累。重组大肠杆菌在较低的比生长速率(μPr约为0.15 h-1)下比在最大比生长速率(μmax = 0.45 h-1)下更有效地表达α1干扰素。因此,在分批培养阶段,仅允许在最大比生长速率下发酵至中等细胞密度。在随后的补料分批培养阶段,根据经验制定的时间尺度,通过提高搅拌器速度将比生长速率降低至μPr。
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