Template:Team:Groningen/CONTENT/EXPERIMENTS/tasA Gel purification (t57)

Afterwards a 1% agarose gel with stain G 1:50000 was run on 100 V for ∼45 minutes. 20 µL of DNA samples were mixed with 4 µL 6x buffer. As a ladder the 10 µL 2log NEB ladder was used. The right bands were cut out, weighed and dissolved in twice as much binding buffer. The samples were purified with the PCR purification kit (Genejet #K0701, lot 00265976) using 25 µL elution buffer. The concentrations were determined with Nanodrop.