Team:The University of Alberta/27 June 2008

Today

 * The O/Ns that were set up last night turned out well. Did mini-preps on them today.
 * The transformations done yesterday turned out perfectly. Now this is what transformations should look like!
 * Running colony PCR as a test for contamination to explain the strange results we got yesterday
 * Gel purified ligations of all the parts we were missing in J61003 (21, 22, 25, 35, 99); also purifying J61003 because we have run out!
 * More transformations: this time on the parts listed above in J61003
 * Made PAGE gels to run the purified His-tagged proteins on.