@article {Cremer2021.01.28.428618, author = {Nils Cremer and Anne Diehl}, title = {Two step PCR method to exchange the resistance cassette of a vector}, elocation-id = {2021.01.28.428618}, year = {2021}, doi = {10.1101/2021.01.28.428618}, publisher = {Cold Spring Harbor Laboratory}, abstract = {For co-transformation of two plasmids, both have to possess different antibiotic selection markers. If that is not the case, normally the gene of interest (GOI) is subcloned into another vector. Here we introduce a fast and easy method to exchange the antibiotic resistance cassette (ARC) in only two PCR steps.Method Summary To shuttle the antibiotic resistance cassette (ARC) from one vector to another, one can amplify the ARC of interest and use the resulting PCR-product as a primer pair for the next amplification step. Simply remove parental DNA template by DpnI digestion, transform PCR product directly in E. coli cells, select transformants on an appropriate agar plate and isolate target vector by plasmid preparation.Competing Interest StatementThe authors have declared no competing interest.}, URL = {https://www.biorxiv.org/content/early/2021/01/28/2021.01.28.428618}, eprint = {https://www.biorxiv.org/content/early/2021/01/28/2021.01.28.428618.full.pdf}, journal = {bioRxiv} }