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Optimization of rPDT fusion protein expression by Escherichia coli in pilot scale fermentation: a statistical experimental design approach

机译:大肠杆菌在中试规模发酵中rPDT融合蛋白表达的优化:统计学实验设计方法

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摘要

High yield recombinant protein production is highly desirable for biotechnological purposes. In the design of recombinant expression conditions, a number of essential central elements such as expression strain, type of medium, bioprocess optimization, and mathematical modeling should be considered. Well-designed industrial scale production of one recombinant protein with optimized influential parameters and yield can address the cost and production reproducibility issues. In the present study, statistical experimental design methodology was used to investigate the effect of fermentation conditions (dissolved oxygen, IPTG, and temperature) on rPDT production by Escherichia coli. rPDT is a recombinant fusion protein consisting of three different protein domains including the N-terminal 179 amino acid fragment of the S1 subunit of pertussis toxin, the full-length genetically detoxified diphtheria toxin (CRM197), and the 50 kDa tetanus toxin fragment C. A 15 Box–Behnken design augmented with center points revealed that IPTG and DO at the center point and low temperature will result in high yield. The optimal condition for rPDT production were found to be 100 µM IPTG, DO 30% and temperature 20 °C.
机译:对于生物技术目的,非常需要高产率的重组蛋白生产。在重组表达条件的设计中,应考虑许多必不可少的核心要素,例如表达菌株,培养基类型,生物工艺优化和数学建模。精心设计的具有最佳影响参数和产量的重组蛋白的工业规模生产可以解决成本和生产可重复性问题。在本研究中,统计实验设计方法用于调查发酵条件(溶解氧,IPTG和温度)对大肠杆菌生产rPDT的影响。 rPDT是一种重组融合蛋白,由三个不同的蛋白结构域组成,包括百日咳毒素的S1亚基的N端179个氨基酸片段,全长的基因解毒白喉毒素(CRM197)和50 kDa的破伤风毒素片段C.具有中心点的15 Box–Behnken设计表明,中心处的IPTG和DO和低温会导致高产量。发现生产rPDT的最佳条件是IPTG 100 µM,DO 30%,温度20°C。

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