November+14-18

November 14, 2011
Today we ran our gel of our GFP and the vector which separated into two linear bands. We then cut them and dissolved them from the gel into pure DNA and vector. media type="custom" key="11325976" media type="custom" key="11325982" These were the instructions for dissoliving the vector and pGlo GFP DNA from the aragose gel media type="custom" key="11325992" And these were our final notes on how to create our own forward and reverse primers of Sma1 and Nhe1