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User:DrJones1935/11 August 2012
From 2012.igem.org
Contents |
I. Ligate Digested Plasmid and Digested Cassette Together
- 1:1 vector:insert ratio - Mix:
- 0.34 uL water
- 2 uL 10X T4 Buffer
- 6 uL plasmid DNA (~0.05 pmol)
- 10.66 uL cassette DNA (~0.05 pmol)
- 1 uL T4 Ligase
- 1:3 vector:insert ratio - Mix:
- 1.2 uL water
- 2 uL 10X T4 Buffer
- 2.5 uL plasmid DNA (~0.0208 pmol)
- 13.30 uL cassette DNA (~0.0624 pmol)
- 1 uL T4 Ligase
- Incubate at room temperature for 10 minutes, then keep on ice
II. Transformation of DH5α Cells with pBAV1K-cassette
- Thaw 5 x50 uL competent DH5α cells on ice
- Add 4 uL of DNA/water according to the following table, swirl gently with pipette
| Name | DNA |
|---|---|
| (-) | water |
| 1:1t | 1:1 ligation |
| 1:1L | 1:1 ligation |
| 1:3t | 1:3 ligation |
| 1:3L | 1:3 ligation |
- Incubate tubes on ice for 30 minutes
- Heat pulse tubes in 42 oC water bath for 40 seconds
- Incubate on ice for 2 minutes
- Transfer cells to 11 mL culture tubes containing 500 uL of LB each, mix gently
- Incubate for an hour at 34 oC with shaking
- Spread with glass beads 100 uL of each culture on an LB agar plate according to the following table and incubate overnight at 34 oC
| Name | Plate |
|---|---|
| (-) | LB + Tetracycline |
| 1:1t | LB + Tetracycline |
| 1:1L | LB |
| 1:3t | LB + Tetracycline |
| 1:3L | LB |
Lab Notes, Sunday, 12 Aug 2012
I. Check Plates for Growth
RESULTS:
Growth on positive controls was a large number of colonies but not a lawn as expected. No growth on any of the Tet50 plates.
II. Streak Out WT ADP1
- Streak ADP1 from glycerol stock onto an LB plate
- Incubate at 34 oC overnight
