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A new and improved host-independent plasmid system for RK2-based conjugal transfer

机译:基于RK2的夫妻转移的新的和改进的主机无关的质粒系统

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摘要

Bacterial conjugation is a process that is mediated either by a direct cell-to-cell junction or by formation of a bridge between the cells. It is often used to transfer DNA constructs designed in Escherichia coli to recipient bacteria, yeast, plants and mammalian cells. Plasmids bearing the RK2/RP4 origin of transfer (oriT) are mostly mobilized using the E. coli S17-1/SM10 donor strains, in which transfer helper functions are provided from a chromosomally integrated RP4::Mu. We have observed that large plasmids were occasionally modified after conjugal transfer when using E. coli S17-1 as a donor. All modified plasmids had increased in size, which most probably was a result of co-transfer of DNA from the chromosomally located oriT. It has earlier also been demonstrated that the bacteriophage Mu is silently transferred to recipient cells by these donor strains, and both occurrences are very likely to lead to mutations within the recipient DNA. Here we report the construction of a new biological system addressing both the above mentioned problems in which the transfer helper functions are provided by a plasmid lacking a functional oriT. This system is compatible with all other replicons commonly used in conjugation experiments and further enables the use of diverse bacterial strains as donors. Plasmids containing large inserts were successfully conjugated and the plasmid modifications observed when E. coli S17-1 was used as donor were eliminated by the use of the new host-independent vector system.
机译:细菌结合是通过直接的细胞间连接或通过细胞之间的桥的形成介导的过程。它通常用于将大肠杆菌中设计的DNA构建体转移到受体细菌,酵母,植物和哺乳动物细胞中。带有RK2 / RP4转移起点(oriT)的质粒大部分是使用大肠杆菌S17-1 / SM10供体菌株动员的,其中从染色体整合的RP4 :: Mu提供转移辅助功能。我们已经观察到,当使用大肠杆菌S17-1作为供体时,大质粒偶尔在接合转移后被修饰。所有修饰的质粒的大小都有所增加,这很可能是DNA从染色体上oriT共转移的结果。早先还证明了噬菌体Mu被这些供体菌株静默转移到受体细胞中,并且两种情况的发生极有可能导致受体DNA内的突变。在这里,我们报告了一个新的生物系统的构建,该系统解决了上述两个问题,其中转移辅助功能由缺乏功能性oriT的质粒提供。该系统与缀合实验中常用的所有其他复制子均兼容,并进一步使得可以使用多种细菌菌株作为供体。成功地缀合了包含大插入片段的质粒,并通过使用新的独立于宿主的载体系统消除了将大肠杆菌S17-1用作供体时观察到的质粒修饰。

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