Team:Paris Saclay/Notebook/July/22
From 2014.igem.org
Contents |
Tuesday 22nd July
Lab Work
A - The chassis coli Odor free
Preparation and transformation of competent cells MG1655 and MG1655Z1
by Arnaud
Dilute 300µl of bacterial culture in 30ml LB medium at 30°C.
Shake vigorously at 30°C until the OD600nm reaches 0,6.
When the OD600 reached 0.6, proceed to the electroporation.
2 - Samples for stock
by Fabio
We collected 1ml of each sample, added 240µl of glycerol (87%) and stored at -80°C.
- BBa_K1033902
- BBa_K1033905
- BBa_K1033910
- BBa_K1033913
- BBa_K1033922
- BBa_K1033925
- BBa_K1033927
- BBa_K1033929
- BBa_K103921
- BBa_J45017
- BBa_K731201
- BBa_K762100
from Liquide Bacterial Cultures transformed the 21st July
3 - Electrophoresis
by Arnaud (Process A), Fabio (gel), Marie and Romain (Process A)
We used 2µL of DNA of the following Biobricks in a 1% Agarose Gel.
Process A
- Empty
- p cola Ges
- DY330 pJBEI I
- DY330 pJBEI II
- BT340
Results:
- A:
4 - Bacterial Culture
by Fabio and Marie
One liquid culture with 5ml of LB (37°C - 150 rpm), IL1403 from the concentrated colony.
5 - Plasmid DNA extraction
by Sean and Terry
Plasmids used: cf part 1
Note: we accidentally used a buffer without 10% ethanol. After removal of the buffer, we repeated the step with a correct version. This may have affected the electrophoresis which followed.
D - Lemon scent
Extraction of p cola plasmid DNA
by Sean
p cola is a low-copy plasmid, and thus requires a slightly different protocol than other plasmids.
PCR Targeting
by Romain
Strains used: DY330 (clone I and II). Plasmid used: pJBEI-6409 (code for enzymes to produce limonene from glucose in E. coli)
Protocol: (For each clone)
Step 1 - Dilution of 300µl of bacterial culture in 30ml of LB + 30µl Cm at 30°C.
Step 2 - With the pre-culture:
- make glycerol stock: 1ml bacterial culture with 240µl glycerol 87%.
- Make extraction of 5ml of plasmid Protocol
Step 3 - When the culture OD650 = 0,6 (Step 1):
- put in ice during 10min.
- centriguge 4°C, 5min, 4000rpm.
- Discard the supernatant, and resuspend the pellet in 30ml glycerol 10% COLD.
- centriguge 4°C, 5min, 4000rpm.
- Discard the supernatant, and resuspend the pellet in 15ml glycerol 10% COLD.
- centriguge 4°C, 5min, 4000rpm.
- Discard the supernatant, and resuspend the pellet in 200µl glycerol 10% COLD.
Step 4 - Transformation:
- control 50µl (without DNA)
- 50µl transformed bacteria + 2,5µl plasmid + 7,5µl pOSV 230 PCR (purifié)
Step 5 - Electroporation control
Step 6 - Spread on ApraR and CmR dishes
- Control dishes : 100µl ND
- 1ml of bacterial culture (250µl on each dish)
Results: 24th July
Reunion
Conference with the team to discuss about the project. The handled topics were:
- Decisions about our new Visual Identity
- Order of the t-shirts and sweaters for the team
- Discussion about the main message of the project
- Presentation's planning of the project
- Exhibition of our draft work
Members there:
- Instructors and advisors: Solenne.
- Students: Arnaud, Fabio, Juliette, Mathieu, Marie, Pierre, Romain, Sean and Terry.