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首页> 外文期刊>Current Microbiology: An International Journal >Efficient Construction of Large Genomic Deletion in Agrobacterium tumefaciens by Combination of Cre/loxP System and Triple Recombineering
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Efficient Construction of Large Genomic Deletion in Agrobacterium tumefaciens by Combination of Cre/loxP System and Triple Recombineering

机译:Cre / loxP系统与三重重组相结合,可有效构建根癌土壤杆菌的大基因组缺失

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摘要

In order to develop an efficient system for deleting genomic segment in Agrobacterium tumefaciens to analyze gene functions and construct marker gene-free recombinant strains, a Cre recombinase expression plasmid was constructed by placing its encoding gene under the control of Ptet promoter and cloning into the plasmid replicable in both A. tumefaciens and E. coli. Triple recombineering was applied to efficiently construct integrative vectors which were used to introduce loxP sites and selection markers into the chromosome of A. tumefaciens. Cre recombinase could be properly induced by anhydrotetracycline in A. tumefaciens, which was revealed by the fact that kanamycin resistance gene flanked by two parallel loxP sites was excised from the genome of A. tumefaciens with virtually 100 % efficiency. And what is more, an A. tumefaciens mutant carrying large-deletion (similar to 85 kb) in genome was successfully constructed by Cre/loxP system. Here, we described the application of combination of Cre/loxP system and triple recombineering to efficiently excise genomic segment in A. tumefaciens, which also would facilitate efficient construction of multiple gene disruptions in A. tumefaciens.
机译:为了开发一种有效的删除根癌土壤杆菌基因组片段以分析基因功能并构建无标记基因重组菌株的系统,通过将其编码基因置于Ptet启动子的控制下并克隆到该质粒中来构建Cre重组酶表达质粒。可在根癌农杆菌和大肠杆菌中复制。三重重组被用于有效地构建整合载体,该整合载体用于将loxP位点和选择标记引入根癌农杆菌的染色体中。 Cre重组酶可以被根癌农杆菌中的脱水四环素适当诱导,这是通过从根癌农杆菌的基因组中切除了两个平行loxP位点的卡那霉素抗性基因这一事实而实现的,其效率几乎为100%。而且,通过Cre / loxP系统成功地构建了在基因组中携带大缺失(类似于85 kb)的根癌农杆菌突变体。在这里,我们描述了Cre / loxP系统和三重重组相结合的应用,以有效地切除根癌农杆菌中的基因组片段,这也将促进根癌农杆菌中多个基因破坏的有效构建。

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