Team:UNIPV-Pavia/Notebook/Week4
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Latest revision as of 21:25, 26 October 2008
Home | The Team | The Project | Biological Safety | Parts Submitted to the Registry |
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Dry Lab | Wet Lab | Modeling | Protocols | Activity Notebook |
Notebook
Week 1 | Week 2 | Week 3 | Week 4 | Week 5 | Week 6 | Week 7 |
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Week 8 | Week 9 | Week 10 | Week 11 | Week 12 | Week 13 | Week 14 |
Week 15 | Week 16 | Week 17 | Week 18 | Week 19 | Week 20 | Week 21 |
Week 22 | Week 23 | Week 24 |
Week 4: 06/09/08 - 06/14/08
06/09/08
- We prepared 4 glycerol stocks taking 800 µl from 9 ml cultures containing:
BBa_B0030 (one of the two cultures) | BBa_R0051 | BBa_E0240 |
BBa_J23100-BBa_B0030 |
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|
- We performed digestion protocol to open plasmids:
BBa_B0030 (1st culture) (E-X) | BBa_R0051 (S-P) | BBa_E0240 (E-X) |
BBa_B0030 (2nd culture) (S-P) |
- We ran a gel with these parts.
- We performed gel extraction.
- Antarctic Phosphatase for these 4 parts.
- Ligation (30 µl final volume):
- BBa_J23100-BBa_E0240 (Pcon(E-S)-assGFP(E-X))
- BBa_R0051-BBa_B0030 (Plam(S-P)-RBS(X-P))
- BBa_B0030-BBa_E0040 (RBS(S-P)-GFP(X-P))
- BBa_B0030-BBa_C0051 (RBS(S-P)-cI(X-P))
- BBa_B0030-BBa_E1010 (RBS(S-P)-RFP(X-P))
- BBa_B0030-BBa_C0061 (RBS(S-P)-luxI_LVA(X-P))
- BBa_B0030-BBa_C0078 (RBS(S-P)-lasI(X-P))
- We incubated ligation overnight at 16°C.
06/10/08
- We transformed the whole volume of the ligations.
- We plated the 7 ligations.
06/11/08
- BBa_J23100-BBa_E0240 and BBa_R0051-BBa_B0030 plates showed respectively 4 and 1 colonies, while the other plates didn't show any colony.
- We picked up one colony from the two working plates to grow 9 ml cultures of transformed bacteria overnight.
- We also infected 9 ml of LB + suitable antibiotic with 30 µl of:
BBa_E0240 | BBa_B0030 | BBa_E0040 | BBa_E1010 |
BBa_C0051 | BBa_C0061 | BBa_C0078 |
- glycerol stocks. We incubated all the 9 ml cultures overnight at 37°C.
- We contacted Francesca Ceroni from Bologna team for suggestions about ligation reaction. We decided to reduce reaction volume from 30 to 20 µl, increment insert:vector molar ratio from 1:2 to 1:3.
06/12/08
- We prepared 9 glycerol stocks taking 800 µl from 9 ml cultures containing:
BBa_E0240 | BBa_B0030 | BBa_E0040 | BBa_R0051-BBa_B0030 |
BBa_C0051 | BBa_C0061 | BBa_C0078 | BBa_J23100-BBa_E0240 |
BBa_E1010 |
- Miniprep for the 9 parts.
- We tested our microscope and BBa_J23100-BBa_E0240 fluorescence:
- We infected 150 µl of LB + Amp with 30 µl of BBa_J23100 glycerol stock (positive control)
- We took 30 µl of BBa_J23100-BBa_E0240 9 ml culture and infected 150 µl of LB + Amp.
- We incubated these two cultures at 37°C, 220 rpm for 3 hours.
- Then, we took the 180 µl cultures and tried to watch them respectively through red and green fluorescence channel. BBa_J23100-BBa_E0240 didn't glow, while our positive control, BBa_J23100, glowed correctly through red channel.
|
- Digestion for:
BBa_E0240 (E-X) | BBa_B0030 (S-P) | BBa_E0040 (X-P) | BBa_E1010 (X-P) |
BBa_C0051 (X-P) | BBa_C0061 (X-P) | BBa_C0078 (X-P) | BBa_J23100 (E-S) |
- Gel run for these parts.
- Gel extraction for these parts.
- Antarctic Phosphatase for BBa_E0240(E-X) and BBa_B0030(S-P)
- Ligation (20 µl final volume):
- BBa_J23100-BBa_E0240 (Pcon(E-S)-assGFP(E-X))
- BBa_B0030-BBa_C0051 (RBS(S-P)-cI(X-P))
- BBa_B0030-BBa_E1010 (RBS(S-P)-RFP(X-P))
- BBa_B0030-BBa_C0061 (RBS(S-P)-luxI_LVA(X-P))
- BBa_B0030-BBa_C0078 (RBS(S-P)-lasI(X-P))
- We prepared 2 eppendorf tubes for each ligation reaction. We incubated one ligation set at 4°C overnight and the other ligation set at 25°C for 3 hours.
- We received sequencing results for BBa_I14032: the sequence was 37 bp long, but it was not PlacIQ. We contacted Meagan to try to solve this problem.
06/13/08
- We prepared 5 glycerol stocks taking 800 µl from 9 ml cultures grown.
- Miniprep for these cultures
- We sent all the 5 purified plasmids to Primm for sequencing.
- We transformed the whole volume of the ligations.
- We plated the 10 ligations.
06/14/08
- Only one of 10 ligation plates worked: BBa_B0030-BBa_C0078 showed one colony...Horrible result!
- We decided to dedicate the following week to debug our protocols and to change something:
- Reduce ligation volume to 10 µl
- Inactivate T4 Ligase after ligation heating at 65°C for 10 min
- Heat at 65°C for 5 min ligation mix before adding T4 Ligase and its buffer
- Use different amounts of vector and insert
- Don't use Antarctic Phosphatase