24 January 2018 1 3K Report

We use iproof polymerase from Bio-Rad and a pair of outward primers to PCR the whole plasmid, then phosphorylate the ends, ligate the PCR product into circular plasmids, and then transform.

It used to work quite efficiently. If the template plasmid has been efficiently removed in DpnI digestion, almost every colony gives the right construct. Lately we observed random deletions at the mutagenesis site at quite high frequency. These are either single nucleotide deletion from either end of the primer, or a deletion of 5-20 nucleotide stretch.

Anyone knows how to fix it? Was it because we switched from phusion to iproof, poor primer quality, poor PCR extension?

Thanks a lot!

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