Optimization of electroporation method and promoter evaluation for type-1 methanotroph, Methylotuvimicrobium alcaliphilum

Shubhasish Goswami, Steven W. Singer, Blake A. Simmons, Deepika Awasthi
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Abstract

Methanotrophic bacteria are promising hosts for methane bioconversion to biochemicals or bioproducts. However, due to limitations associated with long genetic manipulation timelines and, lack of choice in genetic tools required for strain engineering, methanotrophs are currently not employed for bioconversion technologies. In this study, a rapid and reproducible electroporation protocol is developed for type 1 methanotroph, Methylotuvimicrobium alcaliphilum using common laboratory solutions, analyzing optimal electroshock voltages and post-shock cell recovery time. Successful reproducibility of the developed method was achieved when different replicative plasmids were assessed on lab adapted vs. wild-type M. alcaliphilum strains (DASS vs. DSM19304). Overall, a ∼ 3-fold decrease in time is reported with use of electroporation protocol developed here, compared to conjugation, which is the traditionally employed approach. Additionally, an inducible (3-methyl benzoate) and a constitutive (sucrose phosphate synthase) promoter is characterized for their strength in driving gene expression.
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优化 1 型甲烷营养体 Methylotuvimicrobium alcaliphilum 的电穿孔方法和启动子评估
养甲烷细菌是将甲烷生物转化为生物化学品或生物产品的理想宿主。然而,由于遗传操作时间较长以及菌株工程所需的遗传工具缺乏选择等限制,目前还没有将甲烷营养细菌用于生物转化技术。本研究利用普通实验室溶液,为 1 型甲烷营养菌(Methylotuvimicrobium alcaliphilum)开发了一种快速、可重复的电穿孔方案,分析了最佳电击电压和电击后细胞恢复时间。在对实验室适应型与野生型炼藻甲藻菌株(DASS 与 DSM19304)的不同复制质粒进行评估时,成功实现了所开发方法的可重复性。总体而言,与传统的接合法相比,使用电穿孔法的时间缩短了 3 倍。此外,诱导型(3-甲基苯甲酸酯)和组成型(蔗糖磷酸合成酶)启动子在驱动基因表达方面的优势也得到了证实。
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