Colony PCR: Difference between revisions
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Created page with "Reaction mix: H<sub>2</sub>O 16.5 μL 10x Taq/Pfu buffer 2 μL Primer 1 0.4 μL (10 pmol) Primer 2 0.4 μL (10 pmol) dNTP-Mix 0.2 μL Taq polymerase 0.5 μL total ..." |
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Reaction mix | == Reaction mix (Pipett scheme) == | ||
H<sub>2</sub>O 16.5 μL | H<sub>2</sub>O 16.5 μL | ||
Revision as of 15:10, 29 May 2025
Reaction mix (Pipett scheme)
H2O 16.5 μL
10x Taq/Pfu buffer 2 μL
Primer 1 0.4 μL (10 pmol)
Primer 2 0.4 μL (10 pmol)
dNTP-Mix 0.2 μL
Taq polymerase 0.5 μL total 20 μL
| 1 | Innitial melting | 94 ºC | 3 minutes |
| Start-Loop (20x Cycles) | |||
| 2 Denaturation | 94 ºC | 20 seconds | |
| 3 Hybridization | 58 ºC | 20 seconds | |
| 4 Elongation | 72 ºC | 60 seconds per 1000 bp | |
| Close-Loop | |||
| 5 | Elongation | 72 ºC | 5 min |
| 6 | Stop | 8 ºC | |
Procedure
- Prepare a “Chess board” LB-plate of corresponding resistance
- For each colony:
- lightly touch the colony with a yellow pipett-tip, on a 20µl pipett
- Touch a numbered chess-board-tile with a pipett-tip (3 times)
- Place the same tip in a corresponding filled PCR-reaction tube a resuspend 2-3 times
- Run PCR and incubate LB-Plate on 37°C
- Analyse PCR via Gel electrophoresis and identify positive clones
- On the same day positive clones can be expanded from the “Chess board”-LB onto a whole new plate (even if colonies are not yet visible)