Toronto/Lab Protocols/Transformation
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== Transformations == | == Transformations == | ||
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For each plasmid: | For each plasmid: | ||
- | + | # Take competent cells from –80 °C freezer. | |
- | + | # Leave on ice for 10 minutes. | |
- | + | # Add 2-5 μL DNA to competent cell. Remember to label. | |
- | + | # Mix with pipette. | |
- | + | # Sit on ice for 30 minutes. | |
- | + | # Get a beaker of exactly 42 °C water from hot water tap. | |
- | + | # Submerge tubes in hot water for exactly 90 seconds. | |
- | + | # Sit on ice for 5 minutes. | |
- | + | # Add 1 mL of LB. | |
- | + | # Incubate for 1 hour. | |
- | + | # Spread 1 mL on a Petri plate labeled with the appropriate antibiotics. (Dip a glass rod in ethanol and flame it to sterilize, then spread the cells on the plate.) | |
- | + | # Leave the plate with lid half open in the incubator to dry. Rotate the plate 180° every 10 minutes to ensure even spread of bacteria. | |
- | + | # Once dry, turn the plates upside down and incubate overnight. | |
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Back to [[toronto]] | Back to [[toronto]] | ||
Jump to [http://igem.skule.ca/lab/protocols/transformation.htm BlueGenes] | Jump to [http://igem.skule.ca/lab/protocols/transformation.htm BlueGenes] |
Revision as of 03:29, 27 October 2007
Transformations
4 hours
Transformation is a genetic alteration of a cell resulting from the introduction, uptake and expression of foreign genetic material (DNA or RNA). [http://en.wikipedia.org/wiki/Transformation_%28genetics%29 Wikipedia]
Competent cells are bacteria, which can accept extra-chromosomal DNA or plasmids [http://en.wikipedia.org/wiki/Competent_cells Wikipedia].
For each plasmid:
- Take competent cells from –80 °C freezer.
- Leave on ice for 10 minutes.
- Add 2-5 μL DNA to competent cell. Remember to label.
- Mix with pipette.
- Sit on ice for 30 minutes.
- Get a beaker of exactly 42 °C water from hot water tap.
- Submerge tubes in hot water for exactly 90 seconds.
- Sit on ice for 5 minutes.
- Add 1 mL of LB.
- Incubate for 1 hour.
- Spread 1 mL on a Petri plate labeled with the appropriate antibiotics. (Dip a glass rod in ethanol and flame it to sterilize, then spread the cells on the plate.)
- Leave the plate with lid half open in the incubator to dry. Rotate the plate 180° every 10 minutes to ensure even spread of bacteria.
- Once dry, turn the plates upside down and incubate overnight.
Back to toronto
Jump to [http://igem.skule.ca/lab/protocols/transformation.htm BlueGenes]