Copenhagen/2 August 2011

(Difference between revisions)

Latest revision as of 07:36, 3 August 2011

We are very excited about the gel we are going to make today!!

Labwork

Run gel on the PCR products from yesterday - to see if the new primers work better so we now will se an insert. The gel showed a positive result for A1 and A2 in the expr. vector.

Make MiniPrep on the O/N cultures from yesterday which appear to have an insert - we have picked two of each of A1 and A2 which showed a posítive gel result.

Do digestion of PSB1C3 once again, since the digestion O/N was to be in 37 degrees.

PCR on the A1 and B1 from the plates from yesterday - to see if its our procedure thats wrong or there's simply no insert. At the same time we are checking our "old" B1 from the 25/26th of July in the expr. vector: 3 from transformed XLblue cells and 3 colonies from transformed Bl21 cells.

Other work

@@ Line 6: / Line 6: @@
 * Run gel on the PCR products from yesterday - to see if the new primers work better so we now will se an insert. The gel showed a positive result for A1 and A2 in the expr. vector.
+*Image of gel:
+[[image:PCR gel 2-8-11.jpg|400px|right]]
 * Make MiniPrep on the O/N cultures from yesterday which appear to have an insert - we have picked two of each of A1 and A2 which showed a posítive gel result.
@@ Line 11: / Line 16: @@
 * Do digestion of PSB1C3 once again, since the digestion O/N was to be in 37 degrees.
-* PCR on the A1 and B1 from the plates from yesterday - to see if its our´procedure thats wrong or there's simply no insert. At the same time we are checking our "old" B1 in the expr. vector in the PCR.
+* PCR on the A1 and B1 from the plates from yesterday - to see if its our procedure thats wrong or there's simply no insert. At the same time we are checking our "old" B1 from the 25/26th of July in the expr. vector: 3 from transformed XLblue cells  and 3 colonies from transformed Bl21 cells.