Difference between revisions of "Team:IONIS Paris/Notebook"
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<link rel="icon" href="images/favicon.ico" type="image/x-icon"> | <link rel="icon" href="images/favicon.ico" type="image/x-icon"> | ||
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<div class="parallax text-center" style="background-image: url(https://static.igem.org/mediawiki/2015/1/19/NOTE.jpg);"> | <div class="parallax text-center" style="background-image: url(https://static.igem.org/mediawiki/2015/1/19/NOTE.jpg);"> | ||
− | <div class="parallax-pattern-overlay"> | + | <div class="parallax-pattern-overlay" style="height: 100vh; "> |
− | <div class="container text-center" style="height: | + | <div class="container text-center" style="height:600px;padding-top:200px;"> |
<h1 class="intro wow zoomIn" wow-data-delay="0.4s" wow-data-duration="0.9s" style="font-family:sans-serif; color:#B00000 " >Notebook</h1> | <h1 class="intro wow zoomIn" wow-data-delay="0.4s" wow-data-duration="0.9s" style="font-family:sans-serif; color:#B00000 " >Notebook</h1> | ||
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− | + | {{IONIS_Paris/Notebook/18-09-15}} | |
− | + | {{IONIS_Paris/Notebook/17-09-15}} | |
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− | + | {{IONIS_Paris/Notebook/10-09-15}} | |
− | + | {{IONIS_Paris/Notebook/09-09-15}} | |
− | + | {{IONIS_Paris/Notebook/08-09-15}} | |
− | + | {{IONIS_Paris/Notebook/07-09-15}} | |
− | + | {{IONIS_Paris/Notebook/04-09-15}} | |
− | + | {{IONIS_Paris/Notebook/03-09-15}} | |
− | + | {{IONIS_Paris/Notebook/02-09-15}} | |
− | + | {{IONIS_Paris/Notebook/01-09-15}} | |
− | + | {{IONIS_Paris/Notebook/31-08-15}} | |
− | + | {{IONIS_Paris/Notebook/28-08-15}} | |
− | + | {{IONIS_Paris/Notebook/27-08-15}} | |
− | + | {{IONIS_Paris/Notebook/26-08-15}} | |
− | + | {{IONIS_Paris/Notebook/25-08-15}} | |
− | + | {{IONIS_Paris/Notebook/24-08-15}} | |
− | + | {{IONIS_Paris/Notebook/21-08-15}} | |
− | + | {{IONIS_Paris/Notebook/20-08-15}} | |
− | + | {{IONIS_Paris/Notebook/18-08-15}} | |
− | + | {{IONIS_Paris/Notebook/30-07-15}} | |
− | + | {{IONIS_Paris/Notebook/29-07-15}} | |
− | + | {{IONIS_Paris/Notebook/28-07-15}} | |
− | {{IONIS_Paris/ | + | {{IONIS_Paris/Notebook/27-07-15}} |
+ | {{IONIS_Paris/Notebook/22-07-15}} | ||
+ | {{IONIS_Paris/Notebook/17-07-15}} | ||
+ | {{IONIS_Paris/Notebook/16-07-15}} | ||
+ | {{IONIS_Paris/Notebook/15-07-15}} | ||
+ | {{IONIS_Paris/Notebook/10-07-15}} | ||
+ | {{IONIS_Paris/Notebook/09-07-15}} | ||
+ | {{IONIS_Paris/Notebook/08-07-15}} | ||
+ | {{IONIS_Paris/Notebook/07-07-15}} | ||
+ | {{IONIS_Paris/Notebook/06-07-15}} | ||
+ | {{IONIS_Paris/Notebook/03-07-15}} | ||
+ | {{IONIS_Paris/Notebook/01-07-15}} | ||
+ | {{IONIS_Paris/Notebook/30-06-15}} | ||
+ | {{IONIS_Paris/Notebook/12-06-15}} | ||
+ | {{IONIS_Paris/Notebook/11-06-15}} | ||
+ | {{IONIS_Paris/Notebook/10-06-15}} | ||
+ | {{IONIS_Paris/Notebook/09-06-15}} | ||
+ | {{IONIS_Paris/Notebook/05-06-15}} | ||
+ | {{IONIS_Paris/Notebook/04-06-15}} | ||
+ | {{IONIS_Paris/Notebook/02-06-15}} | ||
+ | {{IONIS_Paris/Notebook/29-05-15}} | ||
+ | {{IONIS_Paris/Notebook/28-05-15}} | ||
+ | {{IONIS_Paris/Notebook/26-05-15}} | ||
+ | {{IONIS_Paris/Notebook/25-05-15}} | ||
{{IONIS_Paris/Notebook/22-05-15}} | {{IONIS_Paris/Notebook/22-05-15}} | ||
{{IONIS_Paris/Notebook/21-05-15}} | {{IONIS_Paris/Notebook/21-05-15}} | ||
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<div id="works" class=" clearfix grid"> | <div id="works" class=" clearfix grid"> | ||
− | <figure class="effect-oscar | + | <figure class="effect-oscar" > |
<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/Description" ><figcaption> | |
− | + | <h2>PROJECT</h2> | |
− | <h2> | + | |
<p>Our reality game using bacteria<br> | <p>Our reality game using bacteria<br> | ||
− | + | </p> | |
− | </figcaption> | + | </figcaption></a> |
</figure> | </figure> | ||
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<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 | + | <figure class="effect-oscar"> |
<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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{{IONIS_Paris/FootPage}} | {{IONIS_Paris/FootPage}} | ||
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Latest revision as of 20:46, 18 September 2015
MARCH 2015
APRIL 2015
MAY 2015
JUNE 2015
JULY 2015
AUGUST 2015
SEPT. 2015
Results after PCR from 17/09
Expected results
Results
The band for the third well is good. WE GOT IT !!!!!
Induction of BBa_K325909 and BBa_K1159001 with a solution of arabinose 1%, and a solution of IPTG 1 mM for T7-Nanoluc (should correspond to the effect of a constitutive promoter like T7). Under these conditions, light intensity of T7-nanoluc was 1,2 time higher than the BBa_K1159001.
Effect of the concentration of IPTG inducer to the light intensity of T7-nanoluc part. While the concentration of IPTG does not exceed 1 mM, the light intensity remains low.
Effect of the concentration of arabinose inducer to the light intensity of BBa_K1159001 part. Light intensity is linked to inducer concentration however over 1% of arabinose (final concentration), the intensity not rise anymore.
18 Sept. 15
Miniprep of liquid culture (pSB1C3-Nanoluc)
Digestion of miniprep
Tube | pSB1C3 |
---|---|
H2O MQ | 4 µL |
Buffer 2.1 | 1 µL |
DNA | 3 µL |
EcoRI | 1 µL |
PstI | 1 µL |
37°C, 1h
Expected results
Results
No profile of double digestion for pSB1C3-nanoluc. The third sample looks like a simple digestion PCR checking
- Biobrick quantification for submission:
- Holin/Endolysin reverse: 115 ng/µl
- CCDB reverse: 73 ng/µl
- HOKD reverse: 10 ng/µl
- VVD-YC: 38 ng/µl
- VVD-YN: 37 ng/µl
PCR pSB1C3-NanoLuc
Tube | pSB1C3-NanoLuc (x5) |
---|---|
MQ Water | 40 µL |
RB Buffer | 5 µL |
Mg2+ | 1,5 µL |
dNTP 10 µM | 1 µL |
Primer pSB1C3 Fwd | 1 µL |
Primer pSB1C3 Rev | 1 µL |
DNA | 1 µL |
Taq Pol | 0,5 µL |
37°C, 1h
iGEM TAQ
17 Sept. 15
Miniprep
Liquid culture (pSB1C3-Holin/Endolysin x4 and pSB1C3-pDawn x2)
Liquid culture from the bacterial growth kinetic experiment (pDawn-Holin/Endolysin x2)
Digestion
Tube | Miniprep | pDawn-H/E |
---|---|---|
H2O MQ | 2 μL | 3 μL |
Buffer 2.1 | 1 μL | 1 μL |
DNA | 5 μL | 5 μL |
EcoRI | 1 μL | 1 μL |
PstI | 1 μL | - |
37°C, 1h
Expected results
Results
There were no expected profile of digestion excepted for the first and the third wells with pDawn-Holin/Endolysin.
Digestion
Tube | Biobrick |
---|---|
H2O MQ | 5 μL |
Buffer 2.1 | 1 μL |
DNA | 3 μL |
EcoRI | 1 μL |
37°C, 1h
Liquid culture of bacteria transformed with pSB1C3-nanoluc (x5)
Liquid culture on 96 wells plate
When 0,6 < OD600 < 0,8, induction with arabinose or IPTG
Incubate 5h at 30°C; for BBa_K325909, measure the kinetic during the 5h of induction and take the maximum value
Add 50µL of NanoGlow substrate (Promega) for 50 uL of bacteria
Measure kinetic over 120 min and take maximum value for culture with BBa_K1159001 and T7-nanoluc
16 Sept. 15
Measurement of the OD600 of liquid culture
When the OD600 has reached 0.6 or more, the volume of culture has been divided into 3 erlenmeyers:
1 erlenmeyer without light exposition, 37°C
1 erlenmeyer with light exposition, 37°C
1 erlenmeyer with light exposition, room temperature
Measurement of the OD600 every hour
3 culture on 5have shown a bacterial development
Colony - A6
Colony - A8
Colony - F1
All colonies exhibits same profile under same condition of light exposition and temperature. When the temperature is favorable for a bacterial development, the light activation of pDawn leading to the production of toxin is weak and do not impact a lot the growth of the population of bacteria. But at room temperature (RT°), the induction for protein synthesis is high enough to stop bacterial development
Two things lack to this experiment:
- A longer time to measure if the population of bacteria could really decrease
- A control at room temperature without light exposition to compare it evolution of OD 600 to the grey curve
Digestion
Tube | Miniprep | pSB1C3 iGEM |
---|---|---|
H2O MQ | 4 μL | - |
Buffer 2.1 | 2 μL | 4 μL |
DNA | 3 μL | 30 μL |
EcoRI | 0,5 μL | 3 μL |
PstI | 0,5 μL | 3 μL |
37°C, 1h heat kill: 80°C, 20min
Ligation
Tube | pSB1C3-nanoluc (1:3) | pSB1C3-nanoluc (1:5) |
---|---|---|
H2O MQ | 9 μL | 9,5 μL |
T4 buffer | 2 μL | 2 μL |
pSB1C3 | 5 μL | 5 μL |
NanoLuc | 3 µL (35ng.µL-1) | 2,5 µl (70 ng.µL-1) |
T4 ligase | 1 μL | 1 μL |
Room temperature, 30min heat kill: 65°C, 20min
- Transformation of competent cells with 2 µL of ligation products
Liquid culture
4 colonies from transformation with pSB1C3-Holin/Endolysin
2 colonies from transformation with pSB1C3-pDawn
Transformation
Transformation of competent BL 21(DE3) cells with BBa_K325909, BBa_K1159001 and T7-nanoluc plasmids
15 Sept. 15
PCR Nanoluc
Tube | pSB1C3-Gblock |
---|---|
MQ Water | 40 µL |
RB Buffer | 5 µL |
Mg2+ | 1,5 µL |
dNTP 10 µM | 1 µL |
Primer Fwd | 0,5 µL |
Primer Rev | 0,5 µL |
DNA | 1µL |
Taq Pol | 0,5 µL |
T°C | Time | Cycle | |
---|---|---|---|
Initial denaturation | Denaturation | ||
Annealing | |||
Extension | |||
Final extension | |||
Hold |
PCR colony for pSB1C3-VVD YC + YN and pSB1C3-VVD YN + YC
Tube | pSB1C3-VVD YC + YN (x7) | pSB1C3-VVD YN + YC (x6) |
---|---|---|
MQ Water | 40 µL | 40 µL |
RB Buffer | 5 µL | 5 µL |
Mg2+ | 1,5 µL | 1,5 µL |
dNTP 10 µM | 1 µL | 1 µL |
Primer Fwd | YC Fwd, 0,5 µL | pSB1C3 Fwd 2, 1 µL |
Primer Rev | pSB1C3 Rev 2, 1 µL | YN Rev 1, 0,5 µL |
Taq Pol | 0,5 µL | 0,5 µL |
T°C | Time | Cycle | |
---|---|---|---|
Initial denaturation | Denaturation | ||
Annealing | |||
Extension | |||
Final extension | |||
Hold |
Expected results
Results
Not expected bands for every PCR colony Could be due to the choice of primers
- Make another one with primers for pSB1C3 (more simple)
Digestion
Tube | pSB1C3-pDawn | pSB1C3 iGEM | Nanoluc |
---|---|---|---|
H2O MQ | - | - | 14 μL |
Buffer 2.1 | 1,2 μL | 1,1 μL | 2 μL |
DNA | 10 μL | 8 μL | 2 μL |
Enzyme 1 | XbaI 1 μL | EcoRI 1 μL | EcoRI 1 μL |
Enzyme 2 | - | PstI 1 μL | PstI 1 μL |
37°C, 1h heat kill: 80°C, 20min
Ligation
Tube | pSB1C3-pDawn | pSB1C3-pDawn I-V (1:2) | pSB1C3-pDawn I-V (2:1) | pSB1C3-nanoluc (1:1) | pSB1C3-nanoluc (1:2) |
---|---|---|---|---|---|
H2O MQ | - | - | - | 0,8 μL | 4,3 μL |
T4 buffer | 1,4 μL | - | 0,5 μL | 0,5 μL | 1 μL |
pSB1C3 | - | 1,4 µL | 5,5 µL | 7 µL | 3,5 µL |
Insert | 12,2 μL | 20 μL | 22 μL | 0,7 μL | 0,7 μL |
T4 ligase | 0,5 μL | 1 μL | 1 μL | 0,5 μL | 0,5 μL |
Room temperature, 45min heat kill: 65°C, 20min
- Transformation of competent cells with all ligation products using 1 µL or 3 µL
PCR colony for pSB1C3-VVD YC + YN and pSB1C3-VVD YN + YC
Tube | pSB1C3-VVD YC + YN (x7) | pSB1C3-VVD YN + YC (x7) |
---|---|---|
MQ Water | 40 µL | 40 µL |
RB Buffer | 5 µL | 5 µL |
Mg2+ | 1,5 µL | 1,5 µL |
dNTP 10 µM | 1 µL | 1 µL |
Primer pSB1C3 Fwd | 1 µL | 1 µL |
Primer pSB1C3 Rev | 1 µL | 1 µL |
Taq Pol | 0,5 µL | 0,5 µL |
Expected results
Results
No differences with previous PCR colony
Bands weight do not correspond to the two possible cases “no insertion” or “insertion” of the part
-
Liquid culture of 1 colony of each to analyse the DNA
Bacterial growth kinetic of bacteria transformed with pDawn-H/E
Liquid culture of 100 ml LB + 100 µl Kan for 5 interesting colonies from the experiment of the 09/09
37°C, 120 rpm, O/N, no light exposition
14 Sept. 15
Digestion
Tube | VVD YC | VVD YN |
---|---|---|
H2O MQ | 1 μL | 1 μL |
Buffer 2.1 | 2 μL | 2 μL |
DNA | 15 μL | 15 μL |
Enzyme 1 | EcoRI 1 μL | XbaI 1 μL |
Enzyme 2 | SpeI 1 μL | PstI 1 μL |
37°C, 1h heat kill: 65°C, 20min
Expected results
Results
Ligation
Tube | pSB1C3-VVD YC | pSB1C3-VVD YN | pSB1C3 |
---|---|---|---|
H2O MQ | 2,2 μL | 3,4 μL | 1,8 μL |
T4 ligase buffer | 1 μL | 1 μL | 2 μL |
Insert | VVD YN, 4,1 µL | VVD YC, 2,9 µL | pDawn (28/07), 7,2 µL |
Backbone | 2,2 μL | 2,2 μL | 8 μL |
T4 ligase | 0,5 μL | 0,5 μL | 1 μL |
37°C, 30min heat kill: 65°C, 20min
- Transformation of competent cells with pSB1C3-VVD YC + VVD YN and pSB1C3-VVD YN + VVD YC (1 µL or 4 µL have been used); 30°C all the weekend long
Ligation pDawn Gblock
Tube | pDawn I-II-III | pDawn IV-V |
---|---|---|
T4 ligase buffer | 2 μL | 2,3 μL |
pDawn I | 2,3 μL | - |
pDawn II | 12 μL | - |
pDawn III | 2,7 μL | - |
pDawn IV | - | 13,2 μL |
pDawn V | - | 6,2 μL |
T4 ligase | 1 μL | 1 μL |
Room temperature, 45min heat kill: 65°C, 20min
Purification of pSB1C3-pDawn
20 µL of ligation product + 80 µL of H2O MQ
Add 1/10 (10 µL) of the volume of NaOAc 3M pH 5.2
Add 2,5 volumes (275 µL) of Ethanol 100%
Mix and stored at -20°C for 1 hour at least
Centrifuge 30 sec, 14000 rpm at 4°C
Discard the supernatant
Resuspend the pellet with 500 µL of ethanol 70%, invert up the tube several time
Centrifuge 5 min, 14000 rpm at 4°C
Discard the supernatant and let dry the pellet
Resuspend the pellet with the right amount of water following the final concentration expected (20 µL here)
Ligation pDawn Gblock
Tube | pDawn I-II-III-IV-V |
---|---|
pDawn I-II-III | 20 μL |
pDawn IV-V | 22,3 μL |
T4 ligase | 1 μL |
Room temperature, 45min heat kill: 65°C, 20min
11 Sept. 15
Miniprep of liquid culture (QIAgen kit)
Digestion of miniprep
Tube | Miniprep |
---|---|
H2O MQ | 14 µL |
Buffer 2.1 | 2 µL |
DNA | 3 µL |
EcorI | 0,5 µL |
PstI | 0,5 µL |
37°C, 1h
10 Sept. 15
E.coli DH5 alpha transformation
Transformation of competent cells with pSB1C3-GFP and pSB1C3-H/E (ratio 3:1, 1:1, 1:3) with 3 µl of plasmid.
Liquid cultures on plates from 08/09
Measurements of DO595 and DO405 (wtGFP) all the day long
Typical profile of colonies transformed with pDawn-HOKD under light exposition
Continuous bacterial growth despite light exposure not expected
Typical profile of colonies transformed with pDawn-CCDB under light exposition
Interesting profile with a diminution of the DO595 after it reach 0,6
Typical profile of colonies transformed with pDawn-Holin/Endolysin under light exposition
Continuous bacterial growth in spite of light exposure not expected
But some clones get the following profile
Very interesting profile, the DO600 fall down earlier than for all others clones
Typical profile of colonies transformed with pDawn-GFP under light exposition
Not interesting, all curve are proportional such as there were no production of GFP
PCR colony for pSB1C3-pDawn I-V and pSB1C3-VVD YC-VVD YN
Tube | pSB1C3-pDawn I-V | pSB1C3-VVD YC-VVD YN |
---|---|---|
MQ Water | 40 µL | 40 µL |
RB Buffer | 5 µL | 5 µL |
Mg2+ | 1,5 µL | 1,5 µL |
dNTP 10 µM | 1 µL | 1 µL |
Primer Fwd | pDawn Fwd 2, 0,5 µL | pSB1C3 Fwd 2, 0,8 µL |
Primer Rev | pDawn Rev 2, 0,5 µL | pSB1C3 Rev 2, 0,8 µL |
Taq Pol | 0,5 µL | 0,5 µL |
Expected results
Results
Expected results
Results
No amplification for pSB1C3-pDawn
Soft amplification for pSB1C3-VVD YC-VVD YN 1 only
Several bands (only one expected) and unexpected molecular length for VVD YN, VVD YC, HOKD and CCDB biobricks
Liquid culture
pSB1C3-pDawn, colonies 1 to 5 (there were nothing with PCR colony but we have to try…)
pSB1C3-VVD YC-VVD YN, colony 1
9 September 15
Digestion
Tube | VVD-YC155 | VVD-YN155 |
---|---|---|
Buffer 2.1 | 1.4 µL | 1.4 µL |
DNA | 12 µL | 12 µL |
Enzyme 1 (0,5 µL) | EcoRI | XbaI |
Enzyme 2 (0,5 µL) | SpeI | PstI |
Tube | pSB1C3 | GFP | Holin/Endolysin |
---|---|---|---|
Buffer 2.1 | 1 µL | 1,4 µL | 1,4 µL |
DNA | 8 µL | 12 µL | 12 µL |
EcoRI | 0,5 µL | 0,5 µL | 0,5 µL |
PstI | 0,5 µL | 0,5 µL | 0,5 µL |
37°C, 1h heat kill: 80°C, 20min
Ligation
Tube | pSB1C3-VVD YC-VVD YN |
---|---|
H2O MQ | 0,2 μL |
T4 ligase buffer | 1 μL |
VVD-YC | 2 μL |
VVD-YN | 2,6 μL |
pSB1C3 | 3,7 μL |
T4 ligase | 0,5 μL |
Room temperature, 30 min heat kill: 65°C, 20min
- Transformation of bacteria with 1 µL or 4 µL of pSB1C3-VVD YC-VVD YN
Tube | pSB1C3-GFP | pSB1C3-H/E | |||||
---|---|---|---|---|---|---|---|
Ratio (backbone:insert) |
|
|
|
|
|
|
|
H2O MQ | 6,6 μL | 5,7 μL | 3 μL | 6,4 μL | 5 μL | 0,7 μL | |
T4 ligase buffer | 1 μL | 1 μL | 1 μL | 1 μL | 1 μL | 1 μL | |
Insert | 0,5 μL | 1,4 μL | 4,1 μL | 0,7 μL | 2,1 μL | 6,4 μL | |
pSB1C3 | 1,4 μL | 1,4 μL | 1,4 μL | 1,4 μL | 1,4 μL | 1,4 μL | |
T4 ligase | 0,5 μL | 0,5 μL | 0,5 μL | 0,5 μL | 0,5 μL | 0,5 μL |
Room temperature, 30min heat kill: 65°C, 20min
PCR pSB1C3-Gblock (CCDB, HOKD, VVD YC, VVD YN)
Tube | pSB1C3-Gblock |
---|---|
MQ Water | 40 µL |
RB Buffer | 5 µL |
Mg2+ | 1,5 µL |
dNTP 10 µM | 1 µL |
Primer pSB1C3 Fwd | 1 µL |
Primer pSB1C3 Rev | 1 µL |
DNA | 1µL |
Taq Pol | 0,5 µL |
Cultures from 07/09
Many colonies for pDawn-H/E, pDawn-CCDB, pDawn-HOKD and pDawn-GFP
Few colonies for pSB1C3-pDawn I-V
PCR colonies for pSB1C3-pDawn I-V
Tube | pSB1C3-pDawn I-V |
---|---|
MQ Water | 40 µL |
RB Buffer | 5 µL |
Mg2+ | 1,5 µL |
dNTP 10 µM | 1 µL |
Primer pDawn Fwd 2 | 0,8 µL |
Primer pDawn Rev 2 | 0,8 µL |
Taq Pol | 0,5 µL |
Liquid culture
Liquid culture on 96 wells plates for pDawn-H/E, pDawn-CCDB, pDawn-HOKD and pDawn-GFP:
-
1st plate (for each plasmid) has filled with 250 µL of LB + 25 µL of Kanamycin, 1 well on 2.1 colony / well
Withdraw 125 µL/well and fill the same well of a 2nd plate (save)
Measure the DO595 of 1st plates and let it at 37°C, 120 rpm, O/N with light exposition
8 September 15
Results of transformation from 04/09 (pSB1C3-pDawn I-V)
No colonies
Digestion of pDawn-Gblocks I and V, pDawn and Holin/Endolysin
Tube | pDawn I | pDawn V | pDawn | H/E |
---|---|---|---|---|
Buffer (2 µL) | Cutsmart | Buffer 2.1 | Buffer 2.1 | Buffer 2.1 |
DNA | 12 µL | 12 µL | 12 µL | 12 µL |
Enzyme 1 (0,5 µL) | EcoRI | SphI | EcoRI | EcoRI |
Enzyme 2 (0,5 µL) | SalI | PstI | NheI | SpeI |
Ligation
Tube | pDawn I-II-III |
---|---|
T4 ligase buffer | 1 μL |
pDawn I | 1,8 μL |
pDawn II | 4,6 μL |
pDawn III | 2 μL |
T4 ligase | 0,5 μL |
Tube | pDawn IV-V |
---|---|
T4 ligase buffer | 1,1 μL |
pDawn IV | 5 μL |
pDawn V | 4,6 μL |
T4 ligase | 0,5 μL |
Tube | GFP | Holin/Endolysin | ccdB | HokD |
---|---|---|---|---|
Water | 3,7 µL | 3 µL | 3,3 µL | 4 µL |
T4 ligase Buffer | 1 µL | 1 µL | 1 µL | 1 µL |
pDawn (backbone) | 3,5 µL | 3,5 µL | 3,5 µL | 3,5 µL |
Gblock | 1,3 µL | 2 µL | 1,7 µL | 1 µL |
T4 ligase | 0,5 µL | 0,5 µL | 0,5 µL | 0,5 µL |
Room temperature, 30min heat kill: 65°C, 20min
Tube | pDawn I-V |
---|---|
pDawn I-II-III | 10 μL |
pDawn IV-V | 10 μL |
T4 ligase | 0,5 μL |
Room temperature, 30min heat kill: 65°C, 20min
Tube | pDawn I-V |
---|---|
pDawn I-V | 20 μL |
pSB1C3 | 1 μL |
T4 ligase | 0,5 μL |
Room temperature, 30min heat kill: 65°C, 20min
- Transformation pDawn-Gblocks and pSB1C3-pDawn
7 September 15
Results of liquid cultures
After centrifugation and UV exposure, no green light into the pellet or the supernatant
Liquid culture on plates 96 wells of transformed bacteria with pDawn-toxine (Holin/Endolysin, CCDB, HOKD)
1 colonie / well with 200 µL of LB, 32 wells per type of transformation
37°C, 120 rpm without light exposure
- DO595 to follow bacterial growth under no light exposure condition (no time to switch to light exposure condition and to follow the evolution of the DO595)
Digestion of miniprep from 03/09
Tube | Miniprep |
---|---|
H2O MQ | 2 μL |
Buffer 2.1 | 2 μL |
DNA | 10 μL |
EcoRI | 0,5 μL |
37°C, 1h
Expected results
Results
Bands corresponding to pSB1C3-HOKD and pSB1C3-CCDB seem correct (PCR control required for checking)
About constructions with pDawn, bands at 2100 bp were not expected, and highest bands seem to get the same length require additional tests.
Ligation of pSB1C3 and pDawn Gblocks I-V
Tube | pDawn I-II-III |
---|---|
T4 ligase buffer | 1,3 μL |
pDawn I-V | 12,2 μL |
pSB1C3 | 0,5 μL |
T4 ligase | 0,5 μL |
Room temperature, 30min heat kill: 65°C, 20min
Transformation of 100 µL of competent cells; 30°C during the weekend
Digestion of miniprep from 03/09, pDawn-Gblocks
Tube | Miniprep |
---|---|
H2O MQ | 13 μL |
Buffer 2.1 | 2 μL |
DNA | 4 μL |
EcoRI | 0,5 μL |
EcoRV | 0,5 μL |
37°C, 1h
Expected results
Results
No differences between the four digestion no parts into pDawn
4 September 15
Miniprep on liquid culture
Cf liquid culture of the 02/09/15
Digestion of pDawn I-V purified
Tube | pDawn i-V |
---|---|
Buffer 2.1 | 1,2 µL |
DNA | 10 µL |
EcoRI | 0,5 µL |
PstI | 0,5 µL |
37°C, 1h - heat kill: 80°C, 20min
Liquid culture on plates 96 wells of transformed bacteria with pDawn-GFP
1 colonie / well with 100 µl of LB, 37°C, 120 rpm and light exposition
DO405 and DO595 to determine the presence of GFP Liquid culture into 100 ml Erlenmeyer of the 4 most interesting colonies.
3 September 15
Digestion of miniprep from 01/09 and BBa_K1159001
Tube | Miniprep (01/09) | BBa_K1159001 |
---|---|---|
MQ Water | 12 µL | 12 µL |
Buffer 2.1 | 2 µL | 2 µL |
DNA | 5 µL | 5 µL |
EcoRI | 0,5 µL | 0,5 µL |
PstI | - | 0,5 µL |
BamHI | - | 0,5 µL |
37°C, 1h
Expected results
Results
Interesting band for Construction with VVD YC and VVD YN, require control test;
BBa_K1159001: we get 2 on 3 expected bands, confirmation of the structure of the plasmid with a pBad promoter (not indicated on the registry) before the nanoluc gene.
Liquid culture
pDawn – H/E 20 mL LB + 20 µL Kan, without light;
pDawn – GFP 20 mL LB + 20 µL Kan, with light;
pDawn – HOKD 20 mL LB + 20 µL Kan, without light;
pDawn – CCDB 20 mL LB + 20 µL Kan, without light;
pSB1C3– CCDB;
pSB1C3 – HOKD;
pDawn Gblock I-V purification
10 µl of ligation product + 40 µl of H2O MQ;
Add 1/10 (5µL) of the volume of NaOAc 3M pH 5.2;
Add 2,5 volumes (137,5 µl) of Ethanol 100%;
Mix and stored at -20°C for 1 hour at least;
Centrifuge 30 sec, 14000 rpm at 4°C;
Discard the supernatant;
Resuspend the pellet with 500 µl of ethanol 70%, invert up the tube several time;
Centrifuge 5 min, 14000 rpm at 4°C;
Discard the supernatant and let dry the pellet;
Resuspend the pellet with the right amount of water following the final concentration expected (10µL here)
2 September 15
Digestion pDawn and pDawn Gblocks (I – V)
Tube | pDawn | pDawn I | pDawn II | pDawn III | pDawn IV | pDawn V |
---|---|---|---|---|---|---|
Buffer (2 µL) | Buffer 2.1 | Buffer 3.1 | Cutsmart | Cutsmart | Buffer 2.1 | Buffer 2.1 |
DNA | 12 µL | 12 µL | 12 µL | 12 µL | 12 µL | 12 µL |
Enzyme 1 (0,5 µL) | EcoRI | SalI HF | SalI HF | XmaI | SphI | SphI |
Enzyme 2 (0,5 µL) | PstI | - | XmaI | SphI | - | - |
37°C, 1h heat kill: 80°C, 20min
Expected results
Results
pDawn quantification = 22,8 ng.µL-1
Ligation of Gblocks (GFP, H/E, CCDB, HOKD) into pDawn
Tube | GFP | H/E | ccdB | HokD |
---|---|---|---|---|
Water | 5,1 µL | 4,6 µL | 4,8 µL | 5,3 µL |
T4 ligase Buffer | 1 µL | 1 µL | 1 µL | 1 µL |
pDawn | 0,9 µL | 1,4 µL | 1,2 µL | 0,7 µL |
Plasmid | 2,5 µL | 2,5 µL | 2,5 µL | 2,5 µL |
T4 ligase | 0,5 µL | 0,5 µL | 0,5 µL | 0,5 µL |
Room temperature, 30min heat kill: 80°C, 20min
Transformation of E.coli DH5 alpha competent cells
Dephosphorylation of pDawn IV
Tube | GFP |
---|---|
Cutsmart Buffer | 2 µL |
Plasmid | 15 µL |
rSAP enzyme | 1 µL |
Ligation of pDawn Gblocks
Tube | pDawn I-II-III | pDawn IV-V |
---|---|---|
Water | 4,3 µL | 3,7 µL |
T4 ligase Buffer | 1 µL | 1 µL |
pDawn I | 0,9 µL | - |
pDawn II | 2,3 µL | - |
pDawn III | 2,3 µL | - |
pDawn IV | - | 2,5 µL |
pDawn IV | - | 2,5 µL |
T4 ligase | 0,5 µL | 0,5 µL |
Room temperature, 30min heat kill: 65°C, 20 min
1 September 15
Digestion BBa_K1159001
Tube | BBa_K1159001 |
---|---|
Buffer 2.1 | 2 μL |
DNA | 10 μL |
Enzyme EcoRI | 0,5 μL |
Enzyme PstI | 0,5 μL |
37°C, 1h heat kill: 80°C, 20 min
Expected results
Results
BBa_K1159001: Not expected 1600 bp long band; the sequence of the part did not correspond to information published on the registry
Good amplification of Gblocks fragment (Holin/Endolysin, GFP, VVD YC and VVD YN)
No amplification of HOKD and CCDB fragment
Gel extraction (QIAgen kit)
PCR of Gblocks (CCDB and HOKD)
Gblock | |
---|---|
MQ Water | 39 µL |
RB Buffer | 5 µL |
Mg2+ | 1,5 µL |
dNTP 10 µM | 1 µL |
Primer Fwd 25 µM | 0,5µL pSB1C3 Fwd |
Primer Rev 25 µM | 0,5µL pSB1C3 Rev |
DNA | 1µL |
Taq Pol enzyme | 0,5 µL |
Expected results
Results
Good amplification gel extraction (QIAgen kit)
Liquid culture
2 colonies from culture on plates have been selected for amplification:
VVD YC/YN (x2)
VVD YC (x2)
VVD YN (x2)
GFP (x2)
Holin/Endolysin (x2)
CCDB (x2)
HOKD (x2)pDawn
- 20 ml LB + 20 µl Cam
pDusk
- 20 ml LB + 20 µl Kan
31 August 15
Results
Result of transformation (26/08):
1 colony onto a gel artefact (no antibiotic) of the control plate;
Few colonies (3 to 20) for others plates excepted H/E plates
- Stored into a fridge for WE, H/E plates stayed at room temperature
Miniprep (kit QIAgen)
Liquid culture of bacteria transformed with BBa_K1159001 plasmid (from iGEM) prepared into 2 columns; final elution 2x15µl/column
PCR of Gblocks (VVD YC, VVD YN, GFP, H/E, CCDB and HOKD)
Gblock | |
---|---|
MQ Water | 39 µL |
RB Buffer | 5 µL |
Mg2+ | 1,5 µL |
dNTP 10 µM | 1 µL |
Primer Fwd 25 µM | 1µL pSB1C3 Fwd |
Primer Rev 25 µM | 1µL pSB1C3 Rev |
DNA | 1µL |
Taq Pol enzyme | 0,5 µL |
28 August 15
Digestion
Tube | VVD - YC155 | VVD - YN155 |
---|---|---|
Buffer 2.1 | 2 µL | 2 µL |
DNA | 12 µL | 12 µL |
Enzyme EcoRI | 0,5 µL | - |
Enzyme PstI | - | 0,5 µL |
Enzyme XbaI | - | 0,5 µL |
Enzyme SpeI | 0,5 µL | - |
37°C, 1h heat kill: 80°C, 20 min
Ligation of VVD-YC155 and VVD-YN155 into pSB1C3
Tube | pSB1C3 |
---|---|
Water | 3 µL |
T4 ligase Buffer | 1 µL |
VVD-YC155 | 1,3 µL |
VVD-YN155 | 1,7 µL |
Plasmid | 2,5 µL |
T4 ligase | 0,5 µL |
Room temperature, 30min heat kill: 80°C, 20 min
Transformation of bacteria with ligation products
27 August 15
Digestion of pSB1C3 (from iGEM) and miniprep
Tube | pSB1C3 | pSB1C3 | Miniprep |
---|---|---|---|
Water | 6 µL | 12 µL | 12 µL |
Buffer 2.1 | 4 µL | 2 µL | 2 µL |
Plasmid | 8 µL | 5 µL | 5 µL |
Enzyme EcoRI | 1 µL | - | 0,5 µL |
Enzyme PstI | 1 µL | - | 0,5 µL |
Enzyme XbaI | - | 0,5 µL | - |
Enzyme SpeI | - | 0,5 µL | - |
37°C, 1h
Expected results
Results
There are only bands corresponding to linearized pSB1C3 and one band, unexpected, corresponding to unknown sequence.
PCR of pDawn (1,2,3,4) and VVD-YN (1,2,1/4)
pDawn (1,2,3,4) | VVD-YN (1,2,1/4) | |
---|---|---|
MQ Water | 40 µL | 40 µL |
RB Buffer | 5 µL | 5 µL |
Mg2+ | 1,5 µL | 1,5 µL |
dNTP 10 µM | 1 µL | 1 µL |
Primer Fwd 50 µM | 0,5µL pDawn Fwd I | 0,5µL VVD Fwd I |
Primer Rev 50 µM | 0,5µL pDawn Rev II | 0,5µL YN155 Rev II |
DNA | 1µL | 1µL |
Taq Pol enzyme | 0,5 µL | 0,5 µL |
Ligation of Gblocks into pSB1C3
Tube | VVD-YC155 | VVD-YN155 | GFP rev | H/E rev | CCDB rev | HOKD rev |
---|---|---|---|---|---|---|
Water | 2,4 µL | 1,3 µL | 2,2 µL | - | 3,5 µL | 4,5 µL |
T4 ligase Buffer | 1 µL | 1 µL | 1 µL | 1 µL | 1 µL | 1 µL |
Gblock | 3,6 µL | 4,7 µL | 3,8 µL | 5,8 µL | 2,5 µL | 1,5 µL |
pSB1C3 | 2,5 µL | 2,5 µL | 2,5 µL | 2,5 µL | 2,5 µL | 2,5 µL |
T4 ligase | 0,5 µL | 0,5 µL | 0,5 µL | 0,5 µL | 0,5 µL | 0,5 µL |
Room temperature, 30min
Ligation of pSB1C3 (from iGEM) XbaI-SpeI (circularization)
Tube | pSB1C3 |
---|---|
Water | 3,5 µL |
T4 ligase Buffer | 1 µL |
Plasmid | 5 µL |
T4 ligase | 0,5 µL |
Room temperature, 1h
Expected results
Results
Same band for each sample Impossible Fail
Expected results
Results
Very soft bands at 2000 bp (pSB1C3) and 4000 bp (???)
Some bands between them (apparent on the screen of the gel reader, not on the picture…)
Transformation of bacteria with ligation products
26 August 15
Results of liquid cultures
No bacteria into the control, many bacteria everywhere else
Miniprep (QIAgen)
Digestion of pSB1C3 (from iGEM), miniprep and Gblocks
Miniprep for pDawn and VVD-YN155
Gblocks: ordered fragment from IDT (VVD-YC155, VVD-YN155, GFP rev, Holin/Endolysin rev (H/E rev), CCDB rev, HOKD rev)
Tube | pSB1C3 | Miniprep | Gblocks |
---|---|---|---|
Water | 6 µL | 12 µL | 11 µL |
Buffer 2.1 | 4 µL | 2 µL | 2 µL |
Plasmid | 8 µL | 5 µL | 6 µL |
Enzyme EcoRI | 1 µL | 0,5 µL | 0,5 µL |
Enzyme PstI | 1 µL | 0,5 µL | 0,5 µL |
37°C, 1h heat kill: 80°C, 20min
PCR biobrick pSB1C3_VVD-YC155
VVD-YC155 | |
---|---|
MQ Water | 40 µL |
RB Buffer | 5 µL |
Mg2+ | 1,5 µL |
dNTP 10 µM | 1 µL |
Primer Fwd 50 µM | 0,5µl VVD Fwd I |
Primer Rev 50 µM | 1µl pSB1C3_VVD-YC155 |
Q5 enzyme | 0,5 µL |
T°C | Time | Cycle | |
---|---|---|---|
Initial denaturation | Denaturation | ||
Annealing | |||
Extension | |||
Final extension | |||
Hold |
Expected results
Results
Amplification of VVD-YC155 validation of the biobrick
VVD-YN: bands at 2000 bp only or 2000 bp and 1000 bp (profile of pSB1C3 with RFP) no part
pDawn: bands at 2000 bp only or 2000 bp and 1000 bp (profile of pSB1C3 with RFP) no part
Ligation of Gblocks into pSB1C3
Tube | VVD-YC155 | VVD-YN155 | GFP rev | H/E rev | CCDB rev | HOKD rev |
---|---|---|---|---|---|---|
Water | 9,5 µL | 11,2 µL | 9,5 µL | 12,3 µL | 7 µL | 4,5 µL |
T4 ligase Buffer | 2 µL | 2 µL | 2 µL | 2 µL | 2 µL | 2 µL |
Gblock | 5 µL | 3,3 µL | 5 µL | 2,2 µL | 7,5 µL | 10 µL |
pSB1C3 | 2,5 µL | 2,5 µL | 2,5 µL | 2,5 µL | 2,5 µL | 2,5 µL |
T4 ligase | 1 µL | 1 µL | 1 µL | 1 µL | 1 µL | 1 µL |
Room temperature, 30min
Expected results
Results
Ligation: epic fail
25 August 15
Results of transformations
2 colonies into the negative control plate (satellite colonies?)
Many white and red colonies into other plates (RFP again but not everywhere)
Liquid culture (2 from the negative control, 7 colonies from pDawn plates and 6 from VVD-YN 155 plates).
24 August 15
Expected results
Results
Quantification of pSB1C3: 44,6 ng / µl
Gibson assembly of pDawn and VVD-YN155, NEB kit
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 |
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 | |||||||
pDawnI | |
0.000000067280 | 0.000000031155 | |||||||
pDawn II | |
0.000000094981 | 0.000000031155 | |||||||
pDawn III | |
0.000000112511 | 0.000000031155 |
DNA mix: 1µL of each diluted DNA solution + 6 µL of MQ Water
DNA mix: completed with 10 µL of master mix
50°C, 15min
E.coli transformation: 1 aliquot with 5 µL of assembly product and 1 aliquot with 5 µL of assembly product diluted by a factor 4 for each assembly product, negative control.
30°C during the weekend
21 August 15
Results of transformation with the Gibson assembly products
Red colonies there is still some RFP into the tube with purified/digested pSB1C3
We have to try again
Digestion of pSB1C3
Tube | pSB1C3 |
---|---|
Water | 1,5 µL |
Buffer 2.1 | 5 µL |
Plasmid | 41,5 µL |
Enzyme SpeI | 1 µL |
Enzyme XbaI | 1 µL |
37°C, 120 min --> heat kill: 80°C, 20min
Dephosphorylation of pSB1C3
Tube | pSB1C3 |
---|---|
Cutsmart | 4 µL |
Digested Plasmid | 25 µL |
rSAP | 2 µL |
37°C, 30 min heat kill: 65°C, 5min
Expected results
Results
Incomplete digestion
Excision of 2000bp bands for gel extraction (QIAgen kit)
20 August 15
Assembly of pDawn
Gibson assembly, NEB kit
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 | |
0.000000063713 | 0.000000031857 | |||||||
pDawnI | |
0.000000067280 | 0.000000063713 | |||||||
pDawnII | |
0.000000094981 | 0.000000063713 | |||||||
pDawnIII | |
0.000000112511 | 0.000000063713 |
DNA mix: 1µL of each diluted DNA solution or the indicated volume if no dilution is required (pDawnI) + 6,1 µL of MQ Water
Add 10 µL of master mix
50°C,15min
E.coli transformation: 1 aliquot with 5 µL of assembly product, 1 aliquot with 5 assembly product diluted by a factor 4.
18 August15
pDawn amplification and digestion
PCR2 amplification of pDawn III results
Expected results
Results
Little amplification but not enough
PCR pDawn III
pDawn III | pDawn III | |
---|---|---|
MQ water | 40 µL | 26,5 µL |
RB Buffer | 5 µL | / |
Mg2+ | 1,5 µL | / |
Q5 Buffer | / | 10 µL |
High GC content Buffer | / | 10 µL |
dNTPs 10µM | 1 µL | 1 µL |
Primer Fwd 50µM | 0,5 µL pDawn Fwd VI | 0,5 µL pDawn Fwd VI |
Primer Rev 50µM | 0,5 µL pDawn Rev III-VI | 0,5 µL pDawn Rev III-VI |
DNA | 1µL pDawn III PCR1 | 1µL pDawn III PCR1 |
Taq Pol | 0.5 µL | / |
Q5 Pol | / | 0.5 µL |
T°C | Time | Cycle | |
---|---|---|---|
Initial denaturation | |||
Denaturation | |||
Annealing | |||
Extension | |||
Final extension | |||
Hold |
Expected results
Results
Very good amplification of pDawn III
Gel extraction (kit from QIAgen)
Digestion of pDawn I, II and III
Tube | ||||||||||||
---|---|---|---|---|---|---|---|---|---|---|---|---|
Water | 16 µL | 16 µL | 16 µL | 16 µL | 16 µL | 16 µL | 16 µL | 16 µL | 16 µL | 16 µL | 16 µL | 16 µL |
Buffer 2.1 | 2 µL | 2 µL | 2 µL | / | 2 µL | 2 µL | 2 µL | / | 2 µL | 2 µL | 2 µL | / |
Buffer 3.1 | / | / | / | 2 µL | / | / | / | 2 µL | / | / | / | 2 µL |
DNA | 1,5 µL | 1,5 µL | 1,5 µL | 1,5 µL | 1,5 µL | 1,5 µL | 1,5 µL | 1,5 µL | 1,5 µL | 1,5 µL | 1,5 µL | 1,5 µL |
Enzyme EcoRI | 0,5 µL | / | / | / | 0,5 µL | / | / | / | 0,5µL | / | / | / |
Enzyme XbaI | / | 0,5 µL | / | / | / | 0,5 µL | / | / | / | 0,5 µL | / | / |
Enzyme SpeI | / | / | 0,5 µL | / | / | / | 0,5 µL | / | / | / | 0,5 µL | / |
Enzyme PstI | / | / | / | 0,5 µL | / | / | / | 0,5 µL | / | / | / | 0,5 µL |
37°C, 60 min
Expected results
Results
Simple digestions have shown that no other unexpected restriction site have appeared during PCR amplification of each fragment
30 July 15
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