Difference between revisions of "Team:Paris Saclay/Notebook/September/8"
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(→Q5 PCR on dCas9 ST - GFP 11 in pSB1C3, FRB in pJET and GFP 1.9 in pUC19) |
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Dh5a cells were transformed with pSB1C3 containing FRB - GFP 11, or containing controls (no buffer mix and plasmid alone) using the usual [[Team:Paris_Saclay/Experiments#heat-shocktransformation|protocol]]. As mentioned before, two buffer mix were used. Furthermore, two different DH5a strains were tested (the usual one and another one from Philippe) and at least 12 transformants were cultured overnight : 3 (1 Gibson and 2 controls) x 2 buffer mix x 2 DH5a strains. | Dh5a cells were transformed with pSB1C3 containing FRB - GFP 11, or containing controls (no buffer mix and plasmid alone) using the usual [[Team:Paris_Saclay/Experiments#heat-shocktransformation|protocol]]. As mentioned before, two buffer mix were used. Furthermore, two different DH5a strains were tested (the usual one and another one from Philippe) and at least 12 transformants were cultured overnight : 3 (1 Gibson and 2 controls) x 2 buffer mix x 2 DH5a strains. | ||
| − | ==== | + | ====PCR on FKBP in pJET and gblock 2.2 (part of dCas9 NM - GFP 10) for new clonage strategy ==== |
''By Maxence'' | ''By Maxence'' | ||
| − | Q5 PCR was performed on plasmids with the following protocol | + | An other clonage strategy was performed by using Gibson between FKBP, gblock 2.2 (part of dCas9 NM - GFP 10) and pSB1C3 (the one from dCas9 ST - GFP 11) in order to have FKBP - GFP 10 in pSB1C3. For that purpose, Q5 PCR was performed on plasmids with the following protocol. |
For each 50μl of reaction, mix the following reagents : | For each 50μl of reaction, mix the following reagents : | ||
* 1 µL of plasmid | * 1 µL of plasmid | ||
* 1 µL of dNTPs (10mM) | * 1 µL of dNTPs (10mM) | ||
| − | * | + | * 2.5 µL of each primer mix (10µM) |
* 10 µL of Q5 buffer (5X) | * 10 µL of Q5 buffer (5X) | ||
* 0,5 µL of Q5 high fidelity polymerase | * 0,5 µL of Q5 high fidelity polymerase | ||
| − | * | + | * 32,5 µL of nuclease free water |
Mix gently and aliquot 50 μl of the mix into the PCR tubes on ice. | Mix gently and aliquot 50 μl of the mix into the PCR tubes on ice. | ||
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|- | |- | ||
!Matrix | !Matrix | ||
| − | ! | + | !gblock FKBP in pJET clones 3, 4 and 5 |
| − | + | !gblock 2.2 in pUC19 | |
| − | ! | + | |
|- | |- | ||
|Primers | |Primers | ||
| − | | | + | |iPS145 and iPS146 |
| − | | | + | |iPS147 and iPS84 |
| − | + | ||
|- | |- | ||
|Tm | |Tm | ||
| − | | | + | |62°C |
| − | | | + | |70°C |
| − | + | ||
|- | |- | ||
|t | |t | ||
| − | | | + | |15 sec |
| − | | | + | |15 sec |
|30 sec | |30 sec | ||
|} | |} | ||
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====Colony PCR of 32 clones containing dCas9 NM - GFP 10 in pSB1C3==== | ====Colony PCR of 32 clones containing dCas9 NM - GFP 10 in pSB1C3==== | ||
Revision as of 17:27, 13 September 2016
Contents
- 1 Thursday 8th September
- 1.1 Lab work
- 1.1.1 Visualization
- 1.1.1.1 Gibson of cleaned up PCR products FRB from clone 9 x pSB1C3 - GFP 11 from clone 8
- 1.1.1.2 Transformation of DH5a cells with FRB - GFP 11 in pSB1C3 obtained by Gibson
- 1.1.1.3 PCR on FKBP in pJET and gblock 2.2 (part of dCas9 NM - GFP 10) for new clonage strategy
- 1.1.1.4 Colony PCR of 32 clones containing dCas9 NM - GFP 10 in pSB1C3
- 1.1.1.5 Samples preparation for sequencing
- 1.1.1 Visualization
- 1.1 Lab work
Thursday 8th September
Lab work
Visualization
Gibson of cleaned up PCR products FRB from clone 9 x pSB1C3 - GFP 11 from clone 8
By Maxence
As no colonies were obtained after one night culture, a new Gibson was performed with cleaned up PCR products FRB from clone 9 (insert) x pSB1C3 - GFP 11 from clone 8 (plasmid) (obtained the 6th september) with the following protocol.
Concentration of insert and plasmid were determinated again by Nano drop. For each 20μl of reaction, mix the following reagents :
- 0.65 µL of insert
- 1.1 µL of plasmid
- 8,25 µL of water
- 10 µL of buffer mix
Two controls were done: one without insert and one without buffer (water was added in order to have a total of 20 µL). Two different buffer mix were tested (the usual one and another one from Philippe). The PCR was performed as follow : 1 hour at 50°C.
Transformation of DH5a cells with FRB - GFP 11 in pSB1C3 obtained by Gibson
By Maxence
Dh5a cells were transformed with pSB1C3 containing FRB - GFP 11, or containing controls (no buffer mix and plasmid alone) using the usual protocol. As mentioned before, two buffer mix were used. Furthermore, two different DH5a strains were tested (the usual one and another one from Philippe) and at least 12 transformants were cultured overnight : 3 (1 Gibson and 2 controls) x 2 buffer mix x 2 DH5a strains.
PCR on FKBP in pJET and gblock 2.2 (part of dCas9 NM - GFP 10) for new clonage strategy
By Maxence
An other clonage strategy was performed by using Gibson between FKBP, gblock 2.2 (part of dCas9 NM - GFP 10) and pSB1C3 (the one from dCas9 ST - GFP 11) in order to have FKBP - GFP 10 in pSB1C3. For that purpose, Q5 PCR was performed on plasmids with the following protocol.
For each 50μl of reaction, mix the following reagents :
- 1 µL of plasmid
- 1 µL of dNTPs (10mM)
- 2.5 µL of each primer mix (10µM)
- 10 µL of Q5 buffer (5X)
- 0,5 µL of Q5 high fidelity polymerase
- 32,5 µL of nuclease free water
Mix gently and aliquot 50 μl of the mix into the PCR tubes on ice. Perform PCR as follow:
| Step | Temperature | Time |
|---|---|---|
| Initial denaturation | 98°C | 30sec |
| 30 cycles | 98°C | 10sec |
| Tm | 20sec | |
| 72°C | t | |
| Final Extension | 72°C | 2min |
| Hold | 4°C | $\infty$ |
Primers used were:
| Matrix | gblock FKBP in pJET clones 3, 4 and 5 | gblock 2.2 in pUC19 | |
|---|---|---|---|
| Primers | iPS145 and iPS146 | iPS147 and iPS84 | |
| Tm | 62°C | 70°C | |
| t | 15 sec | 15 sec | 30 sec |
Colony PCR of 32 clones containing dCas9 NM - GFP 10 in pSB1C3
Maxence
Transformed cells which had been grown overnight were used for colony PCR. For that purpose, 16 clones containing dCas9 NM - GFP 10 obtained by Q5 amplification and 16 clones containing dCas9 NM - GFP 10 obtained by Phusion amplification were screened and used for the usual protocol of Colony PCR. The same colonies were also plated on Petri dish containing solid LB + 30 µg/mL Cm and liquid cultures (LB + 30 µg/mL Cm) were made from these clones. Both petri dishes and liquid cultures were grown at 37°C.
For each clones contained in 20 μl water, 4.13 μL of the following mix were added :
- 2.5 µL DreamTaq Buffer
- 0.5 µL of dNTPs (10mM)
- 1 µL of each primer mix (10µM)
- 0.13 μl of DreamTaq Pol
PCR was performed as follow:
| Step | Temperature | Time |
|---|---|---|
| Initial denaturation | 95°C | 3 min |
| 30 cycles | 95°C | 30 sec |
| Tm | 30 sec | |
| 72°C | t | |
| Final Extension | 72°C | 7 min |
| Hold | 4°C | $\infinity\$ |
Primers used were:
| Matrix | Clones containing dCas9 NM - GFP 10 in pSB1C3 |
|---|---|
| Primers | iPS83 and iPS84 |
| Tm | 63.6°C |
| t | 1 min 30 |
After amplification, 3 µL of each PCR products and 5 µL of DNA ladder were placed in wells and migrated at 100V during 30 min.
PCR products expected were :
| PCR products | Expected band size (bp) |
|---|---|
| dCas9 NM - GFP 10 - pSB1C3 | 3688 |
GEL GEL GEL
Samples preparation for sequencing
by Maxence
20 µL of plasmides dCas9 ST - GFP 11 (clones 6 and 8) were sent to be sequenced. 20 µL of the primers iPS168 (5µM), iPS169 (5µM) and iPS171 (5µM) were sent for sequencing.
