Template:Team:KULeuven/7 September 2009/BlueLightReceptor


 * 1) Restriction digest with EcoRI and PstI on  and the purified pcr product of  in order to get our promotor on itself in the  standard vector.
 * 2) Gel electroforesis and extraction of this RD. The concentration of this extraction was too low so no ligation was performed with these samples.
 * 3) Extra pcr was done on  with primers 2260 and 2261.
 * 4) Liquid cultures of LigX and of  were made from the 4x plates.