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Improved method for high-efficiency electrotransformation of Escherichia coli with the large BAC plasmids

机译:大型BAC质粒对大肠杆菌进行高效电转化的改进方法

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High transformation competency of Escherichia coli is one of the critical factors in the bacterial artificial chromosome (BAC)-based DNA library construction. Many electroporation protocols have been published until now, but the majority of them was optimized for transformation of small plasmids. Large plasmids with a size above 50 kbp display reduced transformation efficiency and thereby require specific conditions in the preparation and electroporation of electrocompetent cells. In the present work, we have optimized the parameters critical to the application of BAC DNA electrotransformation into E. coli. Systematic evaluation of electroporation variables has revealed several key factors like temperature of growth, media supplements, washing buffer, and cell concentration. Improvements made in the transformation protocol have led to electrocompetent cells with transformation efficiency up to 7 x 10(8) transformants per microgram of 120 kbp BAC plasmid DNA. We have successfully used in-house prepared competent cells, the quality of which is comparable with those produced by different companies, in the construction of metagenomic libraries from the soil. Our protocol can also be beneficial for other application with limited DNA source.
机译:大肠杆菌的高转化能力是基于细菌人工染色体(BAC)的DNA库构建的关键因素之一。迄今为止,已经发表了许多电穿孔方案,但是其中大多数已针对小质粒的转化进行了优化。大小超过50 kbp的大质粒显示降低的转化效率,因此在制备和感受电感受态细胞时需要特殊条件。在目前的工作中,我们已经优化了对BAC DNA电转化到大肠杆菌中的应用至关重要的参数。对电穿孔变量的系统评估揭示了几个关键因素,例如生长温度,培养基补充剂,洗涤缓冲液和细胞浓度。转化协议中的改进已导致电感受态细胞的转化效率达到每微克120 kbp BAC质粒DNA高达7 x 10(8)个转化子。我们已经成功地使用了内部准备的感受态细胞,其质量与不同公司生产的感受态细胞相当,可用于从土壤中构建宏基因组文库。我们的方案对于DNA来源有限的其他应用也可能是有益的。

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