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Revision as of 11:53, 17 August 2015
PCR VVD BioBricks
PCR.2 VVD - 2nd part
Aim: second step for VVD amplification and mutagenesis
Component | PCR.2 VVD 1 (x2) | PCR.2 VVD 2 (x2) | Control negative | Control negative |
---|---|---|---|---|
DNA Mix "PCR.1 VVD1" | ||||
DNA Mix "PCR.1 VVD2" | ||||
Taq Pol |
Electrophoresis
Aim: check for digestion
1 gel: 120ml TAE 1X + 1,2g agarose + 160µl BET
Sample: 10 µl of PCR product+ 2 µl of loading dye (6x) only 10 µl loaded.
Ladder: 1 µl of 2log ladder (1µg/µl) + 2 µl loading dye (6x) + 9 µl water MQ only 10 µl loaded.
110 V, 30 min
Expected results
Results
We get expected bands about 250 bp meaning DNA have been highly amplified
Purification of PRC product
Aim: purify and concentrate amplified DNA
Use of a QIAquick PCR Purification kit and using a microcentrifuge.
For step 1: add 5 volumes of PB buffer for 1 volume of PCR product
- 200 µl of PB buffer added into both coupled of tube with 40 µl of remaining PCR product
- Mix of same PCR product together into a new tube
- Put mixes into their own purification column
At the end of the purification, we get 1 tube “PCR2, VVD1, 13/05/2015” and another one “PCR2, VVD2, 13/05/2015”
Stored at -20°C.
13 May 15
PCR VVD BioBricks
PCR.1 VVD - 2nd part
Aim: first step for VVD amplification and mutagenesis
Component | PCR.1 VVD 1 (x2) | PCR.1 VVD 2 (x2) |
---|---|---|
PCR mix | ||
Primer VVD Fwd 1 | ||
Primer VVD Rev 1 | ||
Primer VVD Fwd 2 | ||
Primer VVD Rev 2 | ||
Water | ||
Plasmid VVD | ||
Taq Pol |
Electrophoresis
Aim: check for DNA amplification
Low melting point gel
Sample: 10 µl of PCR product+ 2 µl of loading dye (6x)
Ladder: 1 µl of 2log ladder (1µg/µl) + 2 µl of loading dye (6x) + 9 µl water MQ
110 V, 26 min
Expected results
Results
We get expected bands about 200 bp with a good intensity meaning DNA have been highly amplified without contamination.
Purification of PRC product
Aim: purify and concentrate amplified DNA
Use of a QIAquick PCR Purification kit and using a microcentrifuge.
For step 1: add 5 volumes of PB buffer for 1 volume of PCR product
- 200 µl of PB buffer added into both coupled of tube with 40 µl of remaining PCR product
- Mix of same PCR product together into a new tube
- Put mixes into their own purification column
At the end of the purification, we get 1 tube “PCR1, VVD1, 07/05/2015” and another one “PCR1, VVD2, 07/05/2015”
Stored at -20°C.
PCR.2 VVD
Aim: second step for VVD amplification and mutagenesis
dNTP preparation (4µL):
1 µl dATP 100 mM
1 µl dCTP 100 mM
1 µl dTTP 100 mM
1 µl dGTP 100 mM
Store at -20°C
Component | PCR.2 VVD 1 (x2) | PCR.2 VVD 2 (x2) | Control negative (x2) |
---|---|---|---|
Primer VVD Fwd 1 | |||
Primer VVD Rev 3 | |||
Primer VVD Fwd 4 | |||
Primer VVD Rev 2 | |||
Water | |||
Buffer RB | |||
dNTPs | |||
Mg2+ 50mM |
7 May 15
PCR VVD BioBricks
PCR.1 VVD
Aim: first step for VVD amplification and mutagenesis
dNTP preparation (4µL):
1 µl dATP 100 mM
1 µl dCTP 100 mM
1 µl dTTP 100 mM
1 µl dGTP 100 mM
Store at -20°C
T°C | Time | Cycle | |
---|---|---|---|
Initial denaturation | |||
Denaturation | |||
Annealing | |||
Extension | |||
Final extension | |||
Hold |
MQ water | 182,5 µl |
Mg2+ 50 mM | 7,5 µl |
Buffer RB | 25 µl |
dNTPs | 2,5 µl |
Mix preparation for 5 tubes: 43,5 µl / tube
6 May 15
Results
Results from the liquid cultures: all the cultures have grown
Miniprep
Aim: plasmid purification from transformed bacteria
Protocol from MO BIO, UltraClean® Standard
Mini plasmid Prep Kit l
4 plates with Ampicillin
Dilution of the glycerol in water
Percentage in mass not in volume
Ex: 50% glycerol solution 50 g Glycerol + 50 g water (mQ)
Then filtration with vacuum pump
Glycerol preparation & Glycerol Stock
Aim: store the transformed bacteria for later use
Weight 50 g of pure Glycerol
Weight 50 g of distilled water
Mix and homogenize the solution
Filtration with vacuum pump, then close the bottle under PSM
Under PSM class II: put 1ml of liquid culture in a 1,5 ml sterile tube (pDusk, pDawn, psB1C3, VVD)
Centrifugate 1mL of liquid culture 4000 rpm, 5 min
Remove and discard the supernatant
Under PSM: resuspend with 0,5 ml of LB without antibiotics
Add 0,5 ml of glycerol 50% (25% final)
Homogenize
Transfer in an identified cryotube and store at -80°C
1 April 15
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)
Plasmid | Antibiotic | Number of plate | Remarks |
---|---|---|---|
pDusk | |||
Kanamycin | 50 µl of transformed cells | ||
100 µl of transformed cells | |||
50 µl of competent cells (neg control) | |||
pDawn | |||
Kanamycin | 50 µl of transformed cells | ||
100 µl of transformed cells | |||
50 µl of competent cells (neg control) | |||
pSB1C3 | |||
Chloramphenicol | 50 µl of transformed cells | ||
100 µl of transformed cells | |||
50 µl of competent cells (neg control) | |||
VVD | |||
Amplicilin | 50 µl of transformed cells | ||
100 µl of transformed cells | |||
50 µl of competent cells (neg control) | |||
pUC19 | Amplicilin | 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
Tube n° | Reagent added | Volume (µl) | Tube n° | Reagent added | Volume (µl) | ||
---|---|---|---|---|---|---|---|
pDusk | |
pSB1C3 | |
||||
pDawn | |
(Amp control) | |
||||
VVD | |
(Kan control) | |
||||
pUC19 | |
(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
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