Tn5 Transposon-based Mutagenesis for Engineering Phage-resistant Strains of Escherichia coli BL21 (DE3)

大肠杆菌 转座子突变 生物 转座因子 突变 突变体 噬菌体 重组DNA 噬菌体展示 微生物学 噬菌体 表达式向量 拉伤 基因 遗传学 分子生物学 抗体 解剖
作者
Yinfeng Wang,Guanhua Xuan,Houqi Ning,Jiuna Kong,Hong Lin,Jingxue Wang
出处
期刊:Journal of Microbiology [Springer Nature]
卷期号:61 (5): 559-569 被引量:3
标识
DOI:10.1007/s12275-023-00048-2
摘要

Escherichia coli is a preferred strain for recombinant protein production, however, it is often plagued by phage infection during experimental studies and industrial fermentation. While the existing methods of obtaining phage-resistant strains by natural mutation are not efficient enough and time-consuming. Herein, a high-throughput method by combining Tn5 transposon mutation and phage screening was used to produce Escherichia coli BL21 (DE3) phage-resistant strains. Mutant strains PR281-7, PR338-8, PR339-3, PR340-8, and PR347-9 were obtained, and they could effectively resist phage infection. Meanwhile, they had good growth ability, did not contain pseudolysogenic strains, and were controllable. The resultant phage-resistant strains maintained the capabilities of producing recombinant proteins since no difference in mCherry red fluorescent protein expression was found in phage-resistant strains. Comparative genomics showed that PR281-7, PR338-8, PR339-3, and PR340-8 mutated in ecpE, nohD, nrdR, and livM genes, respectively. In this work, a strategy was successfully developed to obtain phage-resistant strains with excellent protein expression characteristics by Tn5 transposon mutation. This study provides a new reference to solve the phage contamination problem.
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