Difference between revisions of "Team:IONIS Paris/Notebook"
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<div id="works" class=" clearfix grid"> | <div id="works" class=" clearfix grid"> | ||
− | <figure class="effect-oscar wowload fadeInUp"> | + | <figure class="effect-oscar wowload fadeInUp" > |
<img src="https://static.igem.org/mediawiki/2015/3/34/Wii.jpg" alt="img01"/> | <img src="https://static.igem.org/mediawiki/2015/3/34/Wii.jpg" alt="img01"/> | ||
− | + | <a href="https://2015.igem.org/Team:IONIS_Paris/Project" ><figcaption> | |
− | <figcaption> | + | <h2>PROJECT</h2> |
− | <h2> | + | |
<p>Our reality game using bacteria<br> | <p>Our reality game using bacteria<br> | ||
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− | </figcaption> | + | </figcaption></a> |
</figure> | </figure> | ||
<figure class="effect-oscar wowload fadeInUp"> | <figure class="effect-oscar wowload fadeInUp"> | ||
<img src="https://static.igem.org/mediawiki/2015/thumb/b/b1/Optogenetics.jpg/800px-Optogenetics.jpg" alt="team"/> | <img src="https://static.igem.org/mediawiki/2015/thumb/b/b1/Optogenetics.jpg/800px-Optogenetics.jpg" alt="team"/> | ||
− | <figcaption> | + | <a href="https://2015.igem.org/Team:IONIS_Paris/Project/Optogenetics" ><figcaption> |
<h2>OPTOGENETICS</h2> | <h2>OPTOGENETICS</h2> | ||
<p>Our scientific core of the project<br> | <p>Our scientific core of the project<br> | ||
− | + | </p> | |
− | </figcaption> | + | </figcaption></a> |
</figure> | </figure> | ||
<figure class="effect-oscar wowload fadeInUp"> | <figure class="effect-oscar wowload fadeInUp"> | ||
<img src="https://static.igem.org/mediawiki/2015/1/18/GRID.jpg" alt="team"/> | <img src="https://static.igem.org/mediawiki/2015/1/18/GRID.jpg" alt="team"/> | ||
− | <figcaption> | + | <a href="https://2015.igem.org/Team:IONIS_Paris/Microfluidics"><figcaption> |
<h2>MICROFLUIDICS</h2> | <h2>MICROFLUIDICS</h2> | ||
<p>Our challenge in achieving the Bio-console<br> | <p>Our challenge in achieving the Bio-console<br> | ||
− | + | </p> | |
− | </figcaption> | + | </figcaption></a> |
</figure> | </figure> | ||
</div> | </div> | ||
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Revision as of 20:26, 7 September 2015
MARCH 2015
APRIL 2015
MAY 2015
JUNE 2015
JULY 2015
AUGUST 2015
SEPT. 2015
Gel extraction of the 3 bands of pDawn
Miniprep of liquid culture with the red colonies
We used a kit from QIAgen
Digestion of pDawn and pSB1C3
Tube | pDawn | Miniprep |
---|---|---|
Water | 12 µL | 12 µL |
Buffer 2.1 | 2 µL | 2 µL |
Plasmid | 5 µL | 5 µL |
Enzyme EcoRI | 0,5 µL | 0,5 µL |
Enzyme SpeI | 0,5 µL | 0,5 µL |
37°C, 60 min
Expected results
Results
We get 2 bands after the digestion of pDawn meaning a non-expected restriction site appeared into the sequence during the PCR useless to answer biobrick standard requirement.
The profile of the Gibson digestion correspond to pSB1C3 with the RFP (totally unexpected since we have purifies the digested backbone).
PCR pDawn III
pDawn III | |
---|---|
MQ water | 26,5 µL |
Q5 Buffer | 10 µL |
High GC content Buffer | 10 µL |
dNTPs 10µM | 1 µL |
Primer Fwd 50µM | 0,5 µL pDawn Fwd VI |
Primer Rev 50µM | 0,5 µL pDawn Rev III-VI |
DNA | 1µL pDawn III PCR1 |
Taq Pol | 0.5 µL |
T°C | Time | Cycle | |
---|---|---|---|
Initial denaturation | |||
Denaturation | |||
Annealing | |||
Extension | |||
Final extension | |||
Hold |
Expected results
Results
There were some amplifications of DNA materials but which one ????
PCR pDawn III
pDawn III | |
---|---|
MQ water | 40 µL |
RB Buffer | 5 µL |
Mg2+ | 1,5 µL |
dNTPs 10µM | 1 µL |
Primer Fwd 50µM | 0,5 µL pDawn Fwd VI |
Primer Rev 50µM | 0,5 µL pDawn Rev III-VI |
DNA | 1µL pDawn III PCR1 |
Taq Pol | 0.5 µL |
T°C | Time | Cycle | |
---|---|---|---|
Initial denaturation | |||
Denaturation | |||
Annealing | |||
Extension | |||
Final extension | |||
Hold |
Digestion of pDawn (PCR and Plasmid)
Tube | pDawn PCR | pDawn PCR | pDawn PCR | pDawn | pDawn |
---|---|---|---|---|---|
Water | 12 µL | 12 µL | 12 µL | 12 µL | 12 µL |
Buffer 2.1 | 2 µL | 2 µL | 2 µL | 2 µL | 2 µL |
Plasmid | 5 µL | 5 µL | 5 µL | 5 µL | 5 µL |
Enzyme EcoRI | 0,5 µL | / | / | 0,5 µL | / |
Enzyme SpeI | / | 0,5 µL | / | / | 0,5 µL |
Enzyme XbaI | / | / | 0,5 µL | / | / |
37°C, 60 min
Expected results
Results
Comparison of digestion profile between the original plasmid and the fragment amplificated by PCR. Confirmation of a new restriction site into pDawn PCR
29 July 15
Results of the last transformation
2 red colonies (which is weird)
Liquid culture for amplification
PCR fragments quantification
Expected results
Results
We get expected bands but, as for second PCRs of VVD and YN155 fragments, bands 2 time heavier than expected bands appeared
Test PCR pDawn (whole fragment)
pDawn (x3) | YC 155 | |
---|---|---|
MQ water | 26,5 µL | 26,5 µL |
Q5 Buffer | 10 µL | 10 µL |
High GC content Buffer | 10 µL | 10 µL |
dNTPs 10µM | 1 µL | 1 µL |
Primer Fwd 50µM | 0,5 µL pDawn Fwd I | 0,5 µL YC155 Fwd |
Primer Rev 50µM | 0,5 µL pDawn Rev III-VI | 0,5 µL YC155 Rev |
DNA | 1µL pDawn | 1µL YC155 PCR1 |
Taq Pol | 0.5 µL | 0.5 µL |
T°C | Time | Cycle | |
---|---|---|---|
Initial denaturation | |||
Denaturation | |||
Annealing | |||
Extension | |||
Final extension | |||
Hold |
Expected results
Results
We get an amplification of pDawn independent of the temperature
Expected results
Results
After the last Gibson reaction we have get red colonies that should correspond to bacteria transformed with pSB1C3-RFP (which should be impossible after the gel migration and purification). So we analyzed the content of the gel extraction and we saw that the tube only had linearized backbone. About pDawn III PCR 2, the migration of 5 µl from the gel extraction of PCR products have shown that there is not a high quantity of DNA material, not enough for a Gibson assembly…
28 July 15
PCR pDawn: whole fragment
pDawn | pDawn | |
---|---|---|
MQ water | 35,5 µL | 35,5 µL |
Q5 Buffer | 10 µL | 10 µL |
High GC content Buffer | / | 10 µL |
dNTPs 10µM | 1 µL | 1 µL |
Primer Fwd 50µM | 1µL pDawn Fwd I | 1µL pDawn Fwd I |
Primer Rev 50µM | 1µL pDawn Rev III-VI | 1µL pDawn Rev III-VI |
DNA | 1µL pDawn | 1µL pDawn |
Taq Pol | 0.5 µL | 0.5 µL |
T°C | Time | Cycle | |
---|---|---|---|
Initial denaturation | |||
Denaturation | |||
Annealing | |||
Extension | |||
Final extension | |||
Hold |
No amplification
Gibson Assembly
Fragments | Concentration (ng.µL-1) | Lenght | Molecular weight (g.mol-1) | Molarity (mol.L-1) | 1/ratio | Dilution factor | Molarity after dilution | DNA Volume | Volume Water | Volume total |
---|---|---|---|---|---|---|---|---|---|---|
pSB1C3 | |
0.000000031155 | 0.000000031155 | |||||||
VVD1 | |
0.000000096698 | 0.000000031155 | |||||||
VVD2 | |
0.000000047103 | 0.000000031155 | |||||||
YN155 I | |
0.000000064805 | 0.000000031155 | |||||||
YN155 II | |
0.000000114117 | 0.000000031155 |
DNA mix:
YN155 1: 1,2µl + 1,3µl of MQ water
YN155 2: 1,2µl + 3,2µl of MQ water
VVD1 : 1µl + 2,1µl of MQ water
VVD2 : 1µl + 0,5 µl of MQ water
pSB1C3 : no dilution
mix= 2µl of each
5µl used for the Gibson assembly added to 15µl of master mix
Transformation of 100 µl of competent cells using 5 µl of Gibson product
27 July 15
Results of bacterial transformation
A total of 12 colonies in both plates containing transformed bacteria
No colony into the negative control
“Biofilm” into the positive control, bacteria are alive and competent
Gel extraction from the cut band of the 16th of July
We used the kit from QIAgen to extract the DNA from the gel
Final elution into 50 µL
Digestion of Gibson product (VVD-YC155)
Tube | Gibson purified |
---|---|
Water | 12 µL |
Buffer 2.1 | 2 µL |
Plasmid | 5 µL |
Enzyme EcoRI | 0,5 µL |
Enzyme PstI | 0,5 µL |
37°C, 60 min
PCR pDawn: whole fragment
pDawn | |
---|---|
MQ water | 35,5 µL |
Q5 Buffer | 10 µL |
dNTPs 10µM | 1 µL |
Primer Fwd 50µM | 1µL pDawn Fwd I |
Primer Rev 50µM | 1µL pDawn Rev III-VI |
DNA | 1µL pDawn |
Taq Pol | 0.5 µL |
T°C | Time | Cycle | |
---|---|---|---|
Initial denaturation | |||
Denaturation | |||
Annealing | |||
Extension | |||
Final extension | |||
Hold |
Electrophoresis of PCR products
Expected results
Results
We get expected bands for our plasmid
No amplification of pDawn
22 July 15