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首页> 外文期刊>Archives of microbiology >'Curing' of plasmid DNA in acetogen using microwave or applying an electric pulse improves cell growth and metabolite production as compared to the plasmid-harboring strain.
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'Curing' of plasmid DNA in acetogen using microwave or applying an electric pulse improves cell growth and metabolite production as compared to the plasmid-harboring strain.

机译:与携带质粒的菌株相比,使用微波或施加电脉冲在丙酮中“固化”质粒DNA可以改善细胞生长和代谢产物的产生。

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Plasmid-free acetogen Clostridium sp. MT962 electrotransformed with a small cryptic plasmid pMT351 was used to develop time- and cost-effective methods for plasmid elimination. Elimination of pMT351 restored production of acetate and ethanol to the levels of the plasmid-free strain with no dry cell weight changes. Destabilizing cell membrane via microwave at 2.45 GHz, or exposure to a single 12 ms square electric pulse at 35 kV cm?1, eliminated pMT351 in 42-47 % of cells. Plasmid elimination with a single square electric pulse required 10 versus 0.1 J needed to introduce the same 3,202-bp plasmid into the cells as calculated per cell sample of Clostridium sp. MT962. Microwave caused visible changes in repPCR pattern and increased ethanol production at the expense of acetate. This is the first report on microwave of microwave ovens, wireless routers, and mobile devices causing chromosomal DNA aberrations in microbes along with carbon flux change.
机译:无质粒的产乙酸梭菌(Clostridium sp。)用小型隐性质粒pMT351电转化的MT962用于开发省时省钱的质粒消除方法。消除pMT351可使乙酸盐和乙醇的产生恢复至无质粒菌株的水平,而干细胞重量无变化。通过在2.45 GHz的微波下使细胞膜失稳,或在35 kV cm?1的单个12 ms方电脉冲下暴露,可以消除42-47%的细胞中的pMT351。用单个方形电脉冲消除质粒需要10到0.1 J,而将相同的3,202 bp质粒引入细胞需要10而不是0.1 J,这是按梭状芽孢杆菌的每个细胞样品计算的。 MT962。微波导致repPCR模式发生明显变化,并以乙酸盐为代价增加了乙醇的产量。这是有关微波炉,无线路由器和移动设备的微波导致微生物染色体DNA畸变以及碳通量变化的第一份报告。

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