Brown: Team Resistance/3 July 2008
From 2008.igem.org
3 July 2008
control: 0.101 (compare 0.054) The pVJ4 cultures with IPTG and the control did not lyse (the OD’s went up slightly at room temperature as expected) The pVJ4 culture with arabinose did lyse (the OD significantly decreased overnight)
Can also load 9ul DNA and 1ul bluejuice depending on desired intensity of band Add 10ul to each well Viewed gel (took picture on gel capture) and saw NO bands Possible that not enough DNA was run in gel, so re-ran gel with 9ul DNA and 1ul bluejuice Still so no bands when gel was viewed Will re-run PCR on sunday with the primers and template primers as a positive control Elongate for 2 minutes Our fragment that we want to amplify is 1320bp without primers. While the 2nd PCR is running, we will digest a microgram of our DNA at sites that are specified in the published sequence of our cassette: EcoRI is found at the beginning EcoRV is found near the middle Therefore, the digested fragment should be approximately 660bp. We will run the digest product alongside our PCR product to ensure that we have the DNA we think we have. Professor Palmore suggested that we use electrodes made of an inert metal i.e. gold or platinum to reduce the possibility of redox chemistry occurring in our solution. We spoke to Mr. Ed Mullen in the machine shop who allowed us to have some platinum wire salvaged from electrophoresis boxes We replaced the copper wire from our old apparatus with platinum wire. |