SBB09Ntbk-Jong H. Shin

Feb 18 2009

First day of the actual lab. Lab work on my project. Template:SBB09 19329 upaG Long I added 275μL of water in the given tube in which JS001F oligo was and 343μL of water in the JS002R tube. Then, I followed the instruction below. Cloning by PCR Since the size is over 4000K, I put the PCR tube in 8k55. Feb 23 2009

Second day of the lab I guess Prof. Chris forgot to give me oligos for Alkaline Phosphatase I should do it later once i get the oligos To decide if there's product in the PCR tube I worked on Feb 18 I need to run it on gel 1. Add 5μL of the product and 1μL of loading buffer 2. Insert 6μL in total onto gel 3. Wait for about 10 minutes 4. GSIs take a picture of my analytical gel 6. The picture link for the first product mine is the 5th one The size is between 1.5k and 1k; it's about the right size I've expected. Product? Yes. The picture link for the second product mine is the 2nd one The result came out the same as the first one. Product? Yes! 7. Zymo cleanup Feb 25 2009

Digestion Regular Zymo cleanup Ligation Mistakes on measuring the volume of the insert PCR again Feb 27 2009

Digestion (upaG) Regular zymo cleanup (upaG) I finally received the oligos for the second part of the project mea36&mea37 1.Dilution 2.Regular PCR  Mar 2-3 2009

Some mistakes occurred on PCR for phoA by GSI Should re-do it Mar 4 2009

upaG Long 1.ligation 2.Accidently put it in the thermalcycler 3.Digestion again 4.Run it on the thermalcycler for about 1 hour phoA 1.Regular PCR again 2.Run on 2k55 since it's under 2k bp (1219bp) Mar 9 2009

upaG Long 1.Ligation The cell cocktail was already set up by GSI Shaking at 37 degree in the incubator 2.  phoA 1.analytical gel The result came out bad-the band of my PCR was overlapped with the bands of ladder Gabe said it would be okay 2.regular zymo cleanup 3.digestion