Multiple site-directed mutagenesis via simple cloning by prolonged overlap extension.

Published in: BioTechniques (2020)

We describe the application of simple cloning by prolonged overlap extension for multiple site-directed mutagenesis in the same plasmid. We show that it is possible to use this technique with very short PCR templates. The technique is ideally suited for the generation of longer donor DNA sequences for CRISPR/Cas9-mediated homologous repair.

Keyphrases

crispr cas
genome editing
circulating tumor
dna damage
single molecule
cell free
oxidative stress
nucleic acid
circulating tumor cells
real time pcr