Bologna University/Transformation
From 2007.igem.org
< Bologna University(Difference between revisions)
| Line 1: | Line 1: | ||
::1. Thaw the competent cells in ice (do not refreeze). | ::1. Thaw the competent cells in ice (do not refreeze). | ||
| - | ::2. Dispense | + | ::2. Dispense 100μl of cells into microfuge tubes on ice. |
| - | ::3. Add 0.1-0. | + | ::3. Add 0.1-0.3μg of plasmidic DNA or the respective amount of the ligation reaction. |
| - | ::4. Keep on ice for | + | ::4. Keep on ice for 30min. |
| - | ::5. Heat at 42 °C for | + | ::5. Heat at 42 °C for 60sec without agitation. |
| - | ::6. Keep on ice for | + | ::6. Keep on ice for 2min. |
| - | ::7. Add 0. | + | ::7. Add 0.9ml of LB medium at room temperature. |
| - | ::8. Incubate at 37 °C for | + | ::8. Incubate at 37 °C for 1hr with agitation. |
| - | ::9. Pellet the cells and discard most of supernatant, leaving about | + | ::9. Pellet the cells and discard most of supernatant, leaving about 100μl. |
::10. Streak on plates containing appropriate antibiotics. | ::10. Streak on plates containing appropriate antibiotics. | ||
::11. Incubate the plates overnight at 37 °C. | ::11. Incubate the plates overnight at 37 °C. | ||
Latest revision as of 09:44, 25 October 2007
- 1. Thaw the competent cells in ice (do not refreeze).
- 2. Dispense 100μl of cells into microfuge tubes on ice.
- 3. Add 0.1-0.3μg of plasmidic DNA or the respective amount of the ligation reaction.
- 4. Keep on ice for 30min.
- 5. Heat at 42 °C for 60sec without agitation.
- 6. Keep on ice for 2min.
- 7. Add 0.9ml of LB medium at room temperature.
- 8. Incubate at 37 °C for 1hr with agitation.
- 9. Pellet the cells and discard most of supernatant, leaving about 100μl.
- 10. Streak on plates containing appropriate antibiotics.
- 11. Incubate the plates overnight at 37 °C.
