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A study of high cell density cultivation process of recombinant Helicobacter pylori multi-epitope vaccine engineering bacteria

机译:重组幽门螺杆菌多表位疫苗工程菌的高细胞密度培养工艺研究

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Objective: To establish high cell density cultivation process of recombinant Helicobacter pylori multi-epitope vaccine engineering bacteria BIB. Methods: Based on the results of shake flask fermentation, the process was magnified into volume of a 50 L fermenter to optimize and verify the factors affecting the yield of the target protein, such as the fermentation medium, working seed inoculation amount, inducer concentration, induction starting time, induction duration, inducer adding mode and feeding strategy. Results: After activated in modified TB medium at 37°C for 8 h, the BIB working seed was inoculated at 5% (v/v) and was induced for expression for another 11 h by the final concentration of 5 mmol/L lactose. In growth phase, glucose at rate of 80 ml/h was used as carbon source, and in induction phase, glycerol at rate of 40 ml/h was used as carbon source; ammonia water was added dropwise to control pH at about 7.0, and revolution speed is adjusted to control the dissolved oxygen at above 30%; ultimately the output of bacterial body was 70 g/L and protein expression amount was about 32%. Conclusion: After high cell density cultivation of the recombinant engineering bacteria, expression and yield of the target protein rBIB significantly increased.
机译:目的:建立重组幽门螺杆菌多表位疫苗工程菌BIB的高细胞密度培养工艺。方法:根据摇瓶发酵的结果,将该过程放大为50 L发酵罐的体积,以优化和验证影响目标蛋白产量的因素,例如发酵培养基,工作种子接种量,诱导剂浓度,诱导开始时间,诱导持续时间,诱导剂添加方式和饲喂策略。结果:在改良的TB培养基中于37℃活化8小时后,以5%(v / v)接种BIB工作种子,并以5 mmol / L的终浓度诱导其再表达11小时。乳糖。在生长期,以80 ml / h的葡萄糖作为碳源,在诱导阶段,以40 ml / h的甘油作为碳源。滴加氨水将pH控制在7.0左右,调节转速使溶解氧控制在30%以上。最终细菌体产量为70 g / L,蛋白质表达量约为32%。结论:重组工程菌经过高细胞密度培养后,靶蛋白rBIB的表达和产量明显增加。

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