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Secretory production of recombinant protein by a high cell density cultureof a protease negative mutant Escherichia coli strain

机译:高细胞密度培养的蛋白酶阴性突变型大肠杆菌菌株分泌重组蛋白

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摘要

Several protease negative mutant strains including HM114, HM126, and HM130 as well as their parent strain KS272 were compared for their growth and secretory production of a model fusion protein, protein A-beta-lactamase. HM114, a strain deficient in two cell envelope proteases, grew slightly faster and produced more fusion protein than the other strains deficient in more proteases. HM114 was grown to a cell dry weight of 47.86 g/L in 29 h using pH-stat, fed-batch cultivation. The beta-lactamase activity was 11.25 x 10(4) U/L, which was 30% higher than that obtained with its parent strain KS272. Up to 96% of protein A-beta-lactamase fusion protein could be recovered by a simple cold osmotic shock method. The specific beta-lactamase activity obtained with HM114 after fractionation was 4.5 times higher than that obtained with KS272.
机译:比较了包括HM114,HM126和HM130在内的几种蛋白酶阴性突变菌株及其亲本菌株KS272,它们的生长和分泌产生了模型融合蛋白,蛋白A-β-内酰胺酶。 HM114是一种缺乏两种细胞包膜蛋白酶的菌株,与其他缺乏更多蛋白酶的菌株相比,其生长速度略快,融合蛋白的产量更高。使用pH固定,分批补料培养,HM114在29小时内生长至细胞干重47.86 g / L。 β-内酰胺酶活性为11.25 x 10(4)U / L,比其亲本菌株KS272获得的活性高30%。通过简单的冷渗透休克方法可以回收多达96%的A-β-内酰胺酶融合蛋白。分馏后,用HM114获得的β-内酰胺酶比活性比KS272获得的高4.5倍。

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