Electrocompetent _E. coli

Making Electocompetent _E. coli Cells

This procedure makes enough electrocompetent cells for 2-3 transformations.

  1. Grow an overnight culture of each strain in LB medium.
  2. Prepare 10 ml of fresh LB medium in a 50 ml flask for each strain.
  3. Inoculate with 100 ul of the overnight, stationary-phase culture.
    • In general, inoculate to OD600 of ~0.05.
  4. Grow the cells for approximately 2-3 hours, until they reach mid-exponential phase.
    • In general, this is an OD600 of ~0.6.
  5. Transfer the cells to 15 ml Falcon conical tubes.
  6. Pellet the cells by centrifugation for 5 minutes at 6,000 RPM. Remove promptly and pour off supernatant.
  7. Wash by adding 10 ml of chilled 10% glycerol to each tube, then vortexing vigorously to resuspend the pellet. Centrifuge for 3.5 minutes. Remove promptly and pour off supernatant. Repeat for at least four wash cycles in 10% glycerol.
  8. Resuspend in approximately 100 µl of 10% glycerol to make a 100x concentration of the initial culture.
  9. Divide into 30-50 µl aliquots in 0.5 or 1.7 ml tubes. Freeze or proceed directly to electroporation.

Notes

  1. Keeping the cells cold during all processing steps is recommended. Ideally, chill the subculture in an ice water bath for >10 min before centrifuging, use a refrigerated centrifuge or a centrifuge in a cold room, and aliquot the final cell slurry into pre-chilled tubes for storage. These precautions are not strictly necessary if using the cells for routine cloning.
  2. Scale up the culture volumes if more electrocompetent cells are needed. The volume of 10% glycerol used for each wash should be at least 20× the volume of the cell pellet.

References

  1. Short Protocols in Molecular Biology, Chapter 1.
  2. Datsenko, K.A., and Wanner, B.L. 2000. One-step inactivation of chromosomal genes in Escherichia coli K-12 using PCR products. Proc. Natl. Acad. Sci. U. S. A. 97: 6640-6645.

Transforming E. coli Cells by Electroporation

This procedure uses the TOP10 Electrocomp™ E. coli cells.

  1. Thaw the electrocompetent cells on ice.
  2. To the electrocompetent cells, add 1-3 μl of DNA (<100 ng of DNA).
  3. Mix by gently flicking the tube containing the electrocompetent cell + DNA mixture. Let the mixture sit on ice for 1-10 minutes.
  4. Pipette the mixture into a chilled cuvette, making sure that the mixture is at the bottom of the cuvette by gently tapping the cuvette on a flat surface.
    • Be sure to wipe any condensation off the sides of the cuvette before electroporation.
  5. Place the cuvette in the pulser and press the "Pulse" button.
    • For the TOP10 Electrocomp™ E. coli cells, the Ecl setting is fine.
  6. After electroporation, add 500-1000 μl of SOC/LB to the cuvette to recover the cells.
  7. Transfer the mixture to a 1.5 mL microcentrifuge tube.
  8. Incubate for ~30-120 minutes at 37°C or other appropriate temperaturein a shaking incubator.
    • Be sure to place the tube on its side so the transformed cells will grow properly.
  9. Plate the cells (~ 50 μl) on an LB plate containing the appropriate antibiotic.
  10. Incubate overnight at 37°C or other appropriate temperature.

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Contributors to this topic Edit topic JeffreyBarrick, KateElston, DanielDeatherage, DaciaLeon, LindseyWolf, AdamHilterbrand, SeanLeonard, JuliePerreau, AlvaroRodriguez
Topic revision: r10 - 2014-05-08 - 17:03:13 - Main.DanielDeatherage
Lab.ProtocolsElectrocompetentCells moved from Lab.ProceduresMakingElectrocompetentCells on 2010-05-07 - 15:02 by Main.JeffreyBarrick -
 
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