Team:BCCS-Bristol/Protocols-Transformation using electroporation
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# Plate a part of the solution or spin the cells down, remove most of the supernatant (800-900 μl), resuspend them and plate all on a LB plate containing antibiotics | # Plate a part of the solution or spin the cells down, remove most of the supernatant (800-900 μl), resuspend them and plate all on a LB plate containing antibiotics | ||
# Incubate the plates overnight at 37°C | # Incubate the plates overnight at 37°C | ||
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Revision as of 19:43, 18 August 2008
Transformation using electroporation
Sterilization of the cuvettes:
- Open the cuvette and put both (lid and cuvette) into a UV light machine (CL-1000 Ultraviolet Crosslinker from UPV)
- Give 1200 “energy” (press “start” and wait for the end of the countdown)
Electroporation
- Prepare 950 μl sterile LB broth in a 1.5 ml tube and put in on ice
- Put the cuvettes at least 2 mins before adding the bacteria on ice
- Thaw the electric competent cells (E. coli DH5α) on ice (here 50 μl cells)
- Add the DNA to the cells (for good working DNA in high concentration like pUC19 with 10 pg/μl use 1 μl; for BioBrick DNA use 5 μl if it was prepared with 10 μl of water)
- Choose program Ec1 (BIORAD MicroPulser) and change the view to “ms” time
- Dry the wet cuvette with a paper towel and put it into the machine
- Give the pulse and notice the time: A pulse between 5-6 ms is a good value
- Add immediately 950 μl ice cold LB broth and transfer everything back into the tube
- Incubate for 1 h at 37°C 225 rpm
- Plate a part of the solution or spin the cells down, remove most of the supernatant (800-900 μl), resuspend them and plate all on a LB plate containing antibiotics
- Incubate the plates overnight at 37°C