A mutagenesis PCR was used to insert a cysteine residue at the C-terminal part of the scaffold His-tag protein.  The correct size of the PCR product was checked via gel electrophoresis. In figure 7 a strong band is visible in the expected height of 6234 bp. The smear above might be the result of an overloaded lane.

The PCR product was self-ligated and E. coli Top 10 cells were transformed with the construct. The PCR product was phosphorylated prior ligation and 2 µL T4 DNA ligase and an incubation time of 2 h were used, additionally. The procedure was adjusted to an online protocol [bitesizebio.com/19149/7-ways-to-improve-blunt-end-ligations (23.07.14)] in order to increase the blunt end ligation efficiency. In the succeeding colony PCR, all five clones showed a positive result of bands migrating at the expected height of 943 bp (see fig 1). Moreover, sequencing of the extracted vectors verified the correct insertion of the cysteine residue in all three chosen clones.