EPF-Lausanne/21 July 2009

  

21 July 2009

Wet Lab
The transformation of the Term plasmids worked, so we did glycerol stocks of the 4 new Term and the death cassette.

Then miniprep of the 5 transformation products.

Digestion following the iGEM protocol : we cut with X and P Term, E and P the backbone and we take a LovTAP that was digested Friday with E and S.

Running of a gel to check the digestion products. Actually it seems the digestion didn't work. We did a second gel, by loading more product, and we clearly got the same result.

As the ligation this way seems not to work (either the enzymes for the digestion aren't working, either there is another problem in the ligation), we decided to try another way to do it : by doing a 2 step PCR. We designed and ordered the primers, now we just have to wait for them to go on in our cloning of LovTAP. Have a look at the cloning strategy to see how we designed the primers.

The idea of [[Media:2step pcr‎.pdf|two step PCR]]

Cloning Strategy
One useful website to know the restriction sites of enzymes: http://www.genscript.com/cgi-bin/products/enzyme.cgi?op=all_ez

The restriction site used were: EcoRI         GAATTC XbaI          TCTAGA SpeI          ACTAGT PsiI          TTATAA

Design the primers for the 2 step-PCR: the first step introduces the LacI promoter and the RBS upstream the LovTAP gene with the Forward primer, whereas the Reverse introduces the Term downstream. In the second step we only introduce the E-X restriction sites upstream and the SP downstream.

People in the lab

 * Nathalie, Caroline, Mélanie, Tu, Heidi

 