Part:BBa_K4687038

MAD7+recE/T+pJYS1+PlacM:MADE/TJlacM-g7

A recombinant plasmid with pJYS1 as the vector backbone, PlacM as the promoter of MAD7, a recE/T recombination system and a gRNA synthesized after a thought-designed design was constructed by utilizing the PCR method as well as a one-step cloning method. Under the action of PlacM promoter, CRISPR-MAD7 gene is expressed, and under the guidance of gRNA, CRISPR-MAD7 can be accurately localized on the target gene for gene editing, and under the action of recE/T recombination system it can help to repair the sheared gene by homologous end recombination. In this study, we combined the recE/T and CRISPR-MAD7 systems. We optimized the MAD7 promoter sequence and selected pJYS1 as the vector backbone for improving the editing efficiency of CRISPR-MAD7 system in Corynebacterium glutamicum.In this study we transferred the constructed recombinant plasmid into E. coli by chemical transformation method to verify the accuracy of the recombinant plasmid. Afterwards, the recombinant plasmid was transferred into Corynebacterium glutamicum by electroporation to observe the colony growth.

Sequence and Features