| Step 1 | Prepare competent cells |
|---|---|
|
Overview Duration |
Grow cells to mid-log and make competent by chemical treatment 3–5 hours |
| 1.1 | Inoculate 100 mls of Psi broth with 0.5 ml of overnight culture and incubate at 37°C with vigorous shaking. |
| 1.2 | When A600 reaches 0.4–0.5 place on ice and chill 5–10 minutes |
| 1.3 | Transfer cells to 50 ml sterile chilled polypropylene centrifuge tubes. Pellet cells at 4°C for 5 minutes at 5,000 × g |
| Tip | If using other tubes they must be very clean and free of soap residue. Cells and transformation buffers should be kept cold at all times. It is also preferable to use chilled pipets and do everything in the cold room if possible. |
| 1.4 | Discard supernatant carefully and gently resuspend cell pellet in 0.4 volume ice cold TfbI (20 mls for each 50 ml tube). Do not vortex and keep on ice while resuspending. |
| 1.5 | Incubate cells on ice for 15 minutes. |
| Tip | Some protocols incubate for only 5 minutes and cells can be left on ice for longer periods (i.e. 1–2 hrs) without any harm |
| 1.6 | Pellet cells at 4°C for 10 minutes at 2,000 × g |
| 1.7 | Discard supernatant carefully and gently resuspend in 0.02 volume (1 ml for 50 mls of culture) TfbII while keeping on ice. |
| 1.8 | Aliquot 50 microliters into 2 ml sterile screw cap tubes with conical bottom and no skirt. Do not use standard 1.5 ml conical microfuge tubes – they don’t work well in the heat shock step of the transformation. |
| 1.9 | Flash freeze in dry ice ethanol bath or liquid nitrogen and store at −80°C |
| Step 2 | Transform competent cells |
|
Overview Duration |
Introduce DNA into competent cells 2 hours |
| 2.1 | Equilibrate a water bath to 42°C. A dry block will work if the tube fits snugly, but is not as good as the water bath. |
| 2.2 | Thaw 1 vial of competent cells on ice for each transformation. Handle gently since cells are sensitive to temperature changes and mechanical lysis. |
| 2.3 | Add 1 to 5 microliters of DNA (10 pg to 100 ng) to a vial of thawed competent cells. DO NOT VORTEX OR PIPETT UP AND DOWN. Supercoiled DNA is transformed more efficiently than ligated DNA. |
| 2.4 | Incubate on ice for 30 minutes |
| 2.5 | Heat shock cells for 30 seconds at 42°C. Do not go any longer or shake the cells |
| 2.6 | Remove from the water bath and place on ice for 2 minutes |
| 2.7 | Add 250 microliters of SOC media to each vial |
| 2.8 | Make sure cap is tight and incubate tube on its side in a 37°C shaking incubator (200–250 rpm) for 1 hour. |
| 2.9 | Spread from 20 – 200 microliters on an appropriate selective plate. The plates should be at room temperature or prewarmed to 37°C. Incubate overnight at 37°C. |
| Tip | Transformed cells can be stored at 4° C for 24–48 hours with minimal loss of viability. Transformation efficiency varies depending on DNA. |
Official websites use .gov
A
.gov website belongs to an official
government organization in the United States.
Secure .gov websites use HTTPS
A lock (
) or https:// means you've safely
connected to the .gov website. Share sensitive
information only on official, secure websites.