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Engineering of a Bacillus amyloliquefaciens Strain with High Neutral Protease Producing Capacity and Optimization of Its Fermentation Conditions

机译:具有高中性蛋白酶生产能力的解淀粉芽孢杆菌菌株的工程设计及其发酵条件的优化

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摘要

The neutral protease has high potential for industrial applications, and attempts to improve enzyme expression level have important application values. In the present study, a neutral protease-encoding gene, Banpr, was cloned from Bacillus amyloliquefaciens strain K11, and a genetic manipulation method specific for this difficult-to-transform strain was developed for the high-level expression of neutral protease. The recombinant plasmid pUB110-Banpr was constructed in Bacillus subtilis strain WB600 and then transformed into strain K11 under optimized conditions. A positive transformant 110N-6 with the highest protease secreting capacity on skim milk plates and great genetic stability for more than 100 generations was selected for further study. Optimization of the fermentation conditions increased the enzyme activity of strain 110N-6 to 8995 ± 250 U/ml in flask culture and 28084 ± 1282 U/ml in 15-l fermentor, which are significantly higher than that of the native strain K11 and industrial strain B. subtilis AS.1398, respectively. The high expression level and extreme genetic stability make B. amyloliquefaciens strain 110N-6 more favorable for mass production of neutral protease for industrial uses.
机译:中性蛋白酶具有工业应用的巨大潜力,并且提高酶表达水平的尝试具有重要的应用价值。在本研究中,从解淀粉芽孢杆菌菌株K11中克隆了一种中性蛋白酶编码基因Banpr,并开发了一种对该难转化菌株特异的遗传操作方法来高水平表达中性蛋白酶。在枯草芽孢杆菌WB600菌株中构建重组质粒pUB110-Banpr,然后在优化条件下转化入菌株K11。选择了在脱脂奶板上具有最高蛋白酶分泌能力且具有超过100代遗传稳定性的正转化体110N-6进行进一步研究。发酵条件的优化使烧瓶培养中的110N-6菌株的酶活性增加到8995±250 U / ml,而在15升发酵罐中的酶活性增加到28084±1282 U / ml,显着高于天然菌株K11和工业菌株。枯草芽孢杆菌菌株AS.1398。高表达水平和极高的遗传稳定性使解淀粉芽孢杆菌菌株110N-6更适合大规模生产工业用途的中性蛋白酶。

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