Repetitive genomic insertion of gene-sized dsDNAs by targeting the promoter region of a counter-selectable marker

نویسندگان

  • Jaehwan Jeong
  • Han Na Seo
  • Yu Kyung Jung
  • Jeewon Lee
  • Gyuri Ryu
  • Wookjae Lee
  • Euijin Kwon
  • Keunsoo Ryoo
  • Jungyeon Kim
  • Hwa-Young Cho
  • Kwang Myung Cho
  • Jin Hwan Park
  • Duhee Bang
چکیده

Genome engineering can be used to produce bacterial strains with a wide range of desired phenotypes. However, the incorporation of gene-sized DNA fragments is often challenging due to the intricacy of the procedure, off-target effects, and low insertion efficiency. Here we report a genome engineering method enabling the continuous incorporation of gene-sized double-stranded DNAs (dsDNAs) into the Escherichia coli genome. DNA substrates are inserted without introducing additional marker genes, by synchronously turning an endogenous counter-selectable marker gene ON and OFF. To accomplish this, we utilized λ Red protein-mediated recombination to insert dsDNAs within the promoter region of a counter-selectable marker gene, tolC. By repeatedly switching the marker gene ON and OFF, a number of desired gene-sized dsDNAs can be inserted consecutively. With this method, we successfully inserted approximately 13 kb gene clusters to generate engineered E. coli strains producing 1,4-butanediol (1,4-BDO).

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عنوان ژورنال:

دوره 5  شماره 

صفحات  -

تاریخ انتشار 2015