Team:EPF Lausanne/Notebook/week2
From 2010.igem.org
(Difference between revisions)
(One intermediate revision not shown) | |||
Line 41: | Line 41: | ||
+ | |||
+ | = Week 2 = | ||
=19-07-2010= | =19-07-2010= | ||
Line 98: | Line 100: | ||
+ | {{EPFL_2010_bottom_wrap}} | ||
</div> | </div> |
Latest revision as of 20:00, 24 October 2010
Contents |
Week 2
19-07-2010
- Results of the transformation checked: successful!!
- Amplification of colonies (goal to do a miniprep of the plasmids --ori-- and --ori-resistance--)
- Results of plating of asaia culture (where we hope to recover the WT) checked: Asaia cultures grew on Kan plates also! Checked colonies for fluorescance under the microscope: no fluorescance --> Very unexpected! Don't know reason yet.
- Re-grow the colonies. Multiple cycles: hope that we get WT.
- Preparation of Asaia cultures for Lemaitre experiments/WT/Competence...
- Preparation of SOC medium and GLY medium
- Autoclaving of media and flasks
20-07-2010
- Plating Asaia to get WT (once again)
- Making HEPES Buffer for the Competence of Asaia
- Diluted the culture to get a 25ml culture(1:20) according to Asaia competence protocol
- OD curve plotted, Doubling time calculated
- No single colonies from the re-growing trial --> replating properly on separate plates
- Preparation of LB medium mixed with Kan/Amp/Cm and GLY medium mixed with <kan
- Miniprep of Origin + Resistance
- Miniprep of Origin alone.
- Miniprep of base vector BBa_151020
- Concentration measurments of miniprep products
- Glycerol stock of BB plasmid and Base Vector made
21-07-2010
- Measure OD of overnight culture of Asaia for competence --> value was too high
- Diluted culture to 0.3 OD, left in 30 degree incubator for 2 hours, OD of 0.6 measured --> start with competence
- Asaia competence
- Digestion of BB's produced and of the Base vector
- Agar plates with Kan/Tet/Cm/Amp made
- Prepared Gel with the products of the digestion to check if the fragments are as expected
- Prepare Tet stock (from powder)
22-07-2010
- Gel with products of digestion run --> only one of the base vector samples and a fragment with the origin and a Kan resistance worked. The others probably did not wok since the concentration of DNA was too low.
- Colonies picked and suspension cultures started. For making a miniprep tomorrow morning.
- Gel cut, Gel purification made
- New idea: PCR run on the product of the miniprep.
- Ligation of Base Vector with Origin+Kan
- Asaia preculture for OD growth (different pH) measurements
- Gly medium with pH 2,3,4,5,6,7.
- Research
- Replating of Asaia (Replating III) to get the WT (one day!!)
23-07-2010
- OD measurement growth curve in function of pH
- new DNA miniprep to extract Ori+AB_Res (the last one failed...)
- Lyse-n-Go protocol to do the ligase (and to check the insertion)
- transformation of the only digestion from yesterday that didn't failed (Kan)
- meeting with Onya for mosquito experiments
- preparation of 4L of Gly for LeMaitre experiments