Dorman:Lambda Red mediated Recombination: Difference between revisions
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Revision as of 10:50, 21 March 2008
We've had trouble getting λ-Red-Mediated recombination to work, but today (21 March 08) finally got it to work well. The protocol below is mostly from Karlinsey (2007). I'll modify/update this as we learn more.
Day 0: Streak out MG1655 w/ pKD46 (you can get this strain from Dan) onto L/Carb and grow o/n at 30°C.
Day 1:
- Pick a single colony off the plate into 1 mL of L in a tube, vortex, and then add the entire volume of this to 25 mL L + 100 μg/mL carbenicillin in a 250 mL flask.
- Grow at 30°C utill the culture reaches an OD600 of between 0.4 to 0.6.
- Add L-arabinose to a final concentration of 0.2% (e.g. 250 μL of 20% arabinose)
- Grow for 1 hour.
- While the cells are inducing, turn on the bucket centrifuge so that it will be at 4°C. Also leave 50 mL of sterile water on ice.
- Take the flasks out of incubator and leave them on an ice/water slurry until the flask is cold. (This took me ~5 min. Remember, an ice/water slurry chills flasks much faster than just ice because the water is a better conductor of heat than air.)
- Transfer the cells into a 50 mL tube, and spin at 4000 rpm in the bucket centrifuge for 7 minutes.
- Pour of the supernatant, add 25 mL of water, and re-suspend by swirling. (You shouldn't need to pipette, and certainly don't vortex!)
- Pellet the cells and repeat the same wash.
- Resuspend the cells in 250 μL of water. They are now ready for electroporation.
- Add 50 μL of cells and 100 to 200 ng of DNA into a 2mm cuvette. Eletroporate at 200Ω, 2.5 kV, and 25 μF.
- Immediately ad 1 mL of L, mix, and pour the entire contents of the cuvette into a 15 mL centrifuge tube.
- Grow for 1 hr with shaking at 37°C.
- Plate 500μL of cells on the appropriate selective media. Leave the rest of the culture to grow o/n in the shaking incubator in case you get no transformants.
Day 3: Hopefully you've got transformants
- Dan Stoebel 12:50, 21 March 2008 (CDT):