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Team:Amsterdam/Notebook/Protocols/ColonyPCR
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=Colony PCR= | =Colony PCR= | ||
| - | We used this protocol to check the new transformants. | + | We used this protocol to check if the new transformants contained the right plasmids/insert. |
==Materials== | ==Materials== | ||
Revision as of 11:56, 19 September 2011
Colony PCR
We used this protocol to check if the new transformants contained the right plasmids/insert.
Materials
- Petri dish with LB agar and appropriate antibiotic
- ON colonies on a petri dish with LB agar and appropriate antibiotic
- dNTPs
- primers ([http://partsregistry.org/Part:BBa_G00100 VF2] and [http://partsregistry.org/Part:BBa_G00101 VR])
- Taq polymerase
- Taq buffer
- dH2O
- PCR tubes
- PCR machine
Protocol
| Sample | µl |
|---|---|
| VF2 primer | 0,5 |
| VR primer | 0,5 |
| dNTPs | 1 |
| Taq buffer | 2,5 |
| Taq polymerase | 0,2 |
| H2O | 20,3 |
| Total | 25 µl |
- Make the PCR mix and pippete it in a PCR tube.
- Pick a colony from a LB-agar plate using a sterile pipette tip.
- Pippete up and down in the PCR mix.
- Cross the pippete tip on the new LB-agar plate in the box corresponding to the sample number.
- Redo this with all the selected colonies.
- Run the following PCR program:
Note: Adjust the elongation time according to the expected product size. 1 minute for each Kb.
- Incubate the selected colonoies on the LB-agar plate ON at 37°C.
- Check the PCR-sample sizes on agarose gel.
