Colony PCR: Difference between revisions

Revision as of 17:38, 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

Thermocycler Protocol

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)

@@ Line 1: / Line 1: @@
-== Reaction mix (Pipett scheme) ==
+{{Minimal-Box
-H<sub>2</sub>O                                         16.5 μL
+|titel=<div>Reaction mix (Pipett scheme)</div>
+|inhalt=
+<div>H<sub>2</sub>O                                         16.5 μL
-x Taq/Pfu buffer                       2 μL
+x Taq/Pfu buffer                    2 μL
 Primer 1                                    0.4 μL (10 pmol)
@@ Line 10: / Line 12: @@
 dNTP-Mix                                  0.2 μL
-Taq polymerase                        0.5 μL total                       20 μL
+Taq polymerase                        0.5 μL total
+<hr style="border: 1px solid #333; margin: 20px 0;">
+μL
+</div>
+}}
+Thermocycler Protocol
 {| class="wikitable"