Team:IONIS Paris/Notebook

Notebook

Results

Results observation for the transformed cells culture (in Petri dishes): no colonies for the positive control pUC19, other plates and negative controls are as expected.

Liquid culture

Antibiotics concentration:
Use of 3 colonies (3 tubes) from VVD, pDawn, pDusk, pSB1C3 3ml LB Broth + 3µl
Antibiotic in double click tubes (12ml) 37°C, 120rpm, O/N



31 March 15

Amplification of pDusk, pDawn, pSB1C3, VVD, pUC19 into E.coli DH5 alpha

Plate preparation

Aim: preparation of selective LB agar plate

Add 50 ml of LB agar into a Falcon tube (50ml) + 50 µl antibiotic
For 25 ml / plate (2 plates)

Agar plates preparation
Plasmid Antibiotic Number of plate Remarks
pDusk
Kanamycin
1
50 µl of transformed cells
1
100 µl of transformed cells
1
50 µl of competent cells (neg control)
pDawn
Kanamycin
1
50 µl of transformed cells
1
100 µl of transformed cells
1
50 µl of competent cells (neg control)
pSB1C3
Chloramphenicol
1
50 µl of transformed cells
1
100 µl of transformed cells
1
50 µl of competent cells (neg control)
VVD
Amplicilin
1
50 µl of transformed cells
1
100 µl of transformed cells
1
50 µl of competent cells (neg control)
pUC19 Amplicilin
1
50 µl of transformed cells

Summary:
6 plates with Kanamycin
3 plates with Chloramphenicol
4 plates with Ampicillin

Antibiotics concentration:
Ampicillin: 50 µg.ml-1 diluted 1/1000
Chloramphenicol: 25 µg.ml-1 diluted 1/1000
Kanamycin: 50 µg.ml-1 diluted 1/1000


Cell transformation

E.coli DH5 alpha (NEB5 alpha competent coli)
Stock: 6 tubes 0.20 ml / tube; 50 pg.µl-1
Aliquot of 50 µl of competent E.coli / transformation

Into aliquots, added plasmids or nothing (control) as following:
Tube n° Reagent added Volume (µl) Tube n° Reagent added Volume (µl)
1
pDusk
1
5
pSB1C3
1
2
pDawn
1
6
(Amp control)
/
3
VVD
1
7
(Kan control)
/
4
pUC19
1
8
(Cam control)
/

Incubation on ice, 30 min
Heat shock exactly 42°C, 30 seconds. Do not mix
Keep on ice for 5 min, do not mix
400 µl of LB in sterile condition without antibiotic, pipette up and down gently
Incubation 37°C, 120 rpm, 1 hour
Centrifuge, 4000 rpm, 5 min
Remove and discard 300 µl of supernatant; resuspend gently using a pipette the remaining 150 µl
Plate bacteria following the table about plate preparation
Incubate at 37°C, O/N

Expected results:
No colonies into the 3 control plates
Many colonies into all the other plates;
Colonies from pSB1C3 transformation should exhibit red color


30 March 15

Preparation of media

Aim: prepare media for bacteria culture
For 250mL
LB Broth LB Agar
2.5g tryptone 2.5g tryptone
2.5g NaCl 2.5g NaCl
1.25g yeast extract 1.25g yeast extract
5.0g agar

Qsp 250 ml distilled water
2 bottles of LB broth and 2 bottles of LB agar (+magnetic stirrer)
Auctoclave 121°C



28 March 15
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