"
Team:DTU-Denmark/Notebook/10 July 2013
From 2013.igem.org
(Difference between revisions)
(→Results) |
(→Results) |
||
| Line 103: | Line 103: | ||
*6: Nir from purification of 08.07.2013 | *6: Nir from purification of 08.07.2013 | ||
*7: Broadband Ladder | *7: Broadband Ladder | ||
| - | *8: Nir from purification | + | *8: Nir from purification of 09.07.2013 |
| - | *9: | + | *9: Nir from purification of 09.07.2013 |
| + | *10: Nir from purification of 09.07.2013 | ||
| + | |||
[[File:2013_07_10_gel_nir.jpg |600px]] | [[File:2013_07_10_gel_nir.jpg |600px]] | ||
Revision as of 12:19, 11 July 2013
Contents |
208
Main purpose
Run gel with 9 PCR samples of Nir operon from Pseudomonas aeruginosa
Transformation of Biobricks
PCR reaction for Nir operon
Who was in the lab
Ariadni,Henrike,Julia,Natalia
Procedure
Run gel
- 3 samples from PCR of 09.07.2013
- 3 samples from PCR purification of 08.07.2013
- ladder broadband
- 3 samples from purification of 09.07.2013
Transformation of Biobricks
According to the iGEM protocol ([http://parts.igem.org/Help:Protocols/Transformation transformation protocol]) with slight changes.
- step 1: 100 μl cells
- step 2: 1.5 μl of the resuspended DNA
- step 6: 90 sec (instead of 60 s)at 42 oC
- step 9: Incubation without shaking
Transformation list
| BioBrick number | Backbone | Resistance | Plate | Well | Copies |
|---|---|---|---|---|---|
| J04450 | pSB3C5 | CAM | 2 | 4D | 10-12 |
| J04450 | pSB4C5 | CAM | 2 | 4F | 5 |
| J04450 | pSB4K5 | Kan | 2 | 6H | 5 |
| J04450 | pSB1T3 | Tetra | 2 | 8B | 100-300 |
| J04450 | pSB3T5 | Tetra | 2 | 8D | 10-12 |
| J04450 | pSB1AK3 | Amp+Kan | 2 | 12B | 100-300 |
| J04450 | pSB1A3 | Amp | 2 | 2H | 100-300 |
| J04450 | pSB1A2 | Amp | 5 | 1B | 100-300 |
| J04450 | pSB6A1 | Amp | 5 | 1K | 10-15 |
| J04450 | pSB1K3 | Kan | 5 | 5A | 100-300 |
| J04450 | pSB3K3 | Kan | 5 | 5E | 10-12 |
| K325909 | pSB1C3 | CAM | 1 | 4L | 100-300 |
| K325209 | pSB1C3 | CAM | 1 | 12H | 100-300 |
| K325219 | pSB1C3 | CAM | 1 | 2D | 100-300 |
| J04421 | pSB1C3 | CAM | 3 | 15O | 100-300 |
| E0430 | pSB1C3 | CAM | 3 | 20K | 10-300 |
Extraction PCR
9 samples from culture pAO1 10 reactions
- dNTP: 1 ul (10 ul)
- HF buffer: 10 ul (100 ul)
- Phusion polymerase: 0.5 ul (5 ul)
- H2O: 31.5 ul (315 ul)
Settings for PCR with three different elongation times
| Temperature (oC) | Time (min) | Rounds |
|---|---|---|
| 98 | 2:00 | 1 |
| 98 | 0:20 | 35 |
| 66 | 0:45 | 35 |
| 72 | 2:00/3:00/4:00 | 35 |
| 72 | 5:00 | 1 |
| 4 | ∞ | - |
Results
0.8 % Agorase Gel (Nir operon)
Wells
- 1: Nir from culture PAO1
- 2: Nir from culture PAO1
- 3: Nir from culture PAO1
- 4: Nir from purification of 08.07.2013
- 5: Nir from purification of 08.07.2013
- 6: Nir from purification of 08.07.2013
- 7: Broadband Ladder
- 8: Nir from purification of 09.07.2013
- 9: Nir from purification of 09.07.2013
- 10: Nir from purification of 09.07.2013
Comments
Kanamycin plates were of bad quality
Tetracyclin plates were made by adding 22.5 uL of tetracyclin stock to LB plates
- Stock tetracyclin: 10 mg/mL
- Final concentration in plates: 15 ug/mL
