Difference between revisions of "Team:Paris Saclay/Notebook/September/7"
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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 [[Team:Paris_Saclay/Experiments##Polymerase_chain_reaction|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. | 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 [[Team:Paris_Saclay/Experiments##Polymerase_chain_reaction|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 50μl of reaction, mix the following reagents : | ||
| + | * 1 µL of plasmid | ||
| + | * 1 µL of dNTPs (10mM) | ||
| + | * 1 µL of each primer mix (10µM) | ||
| + | * 10 µL of Q5 buffer (5X) | ||
| + | * 0,5 µL of Q5 high fidelity polymerase | ||
| + | * 35,5 µL of nuclease free water | ||
| + | |||
| + | Mix gently and aliquot 50 μl of the mix into the PCR tubes on ice. | ||
| + | Perform PCR as follow: | ||
| + | {| class="wikitable" | ||
| + | |- | ||
| + | !Step | ||
| + | !Temperature | ||
| + | !Time | ||
| + | |- | ||
| + | |Initial denaturation | ||
| + | |98°C | ||
| + | |30sec | ||
| + | |- | ||
| + | |rowspan="3"|30 cycles | ||
| + | |98°C | ||
| + | |10sec | ||
| + | |- | ||
| + | |Tm | ||
| + | |20sec | ||
| + | |- | ||
| + | |72°C | ||
| + | |t | ||
| + | |- | ||
| + | |Final Extension | ||
| + | |72°C | ||
| + | |2min | ||
| + | |- | ||
| + | |Hold | ||
| + | |4°C | ||
| + | |$\infinity\$ | ||
| + | |} | ||
| + | |||
| + | [[Team:Paris_Saclay/Experiments#primers|Primers]] used were: | ||
| + | |||
| + | {| class="wikitable" | ||
| + | |- | ||
| + | !Matrix | ||
| + | !dCas9 ST - GFP 11 in pSB1C3 clones 6 and 8 | ||
| + | !FRB in pJET clones 4 and 9 | ||
| + | !GFP 1.9 in pUC19 | ||
| + | |- | ||
| + | |Primers | ||
| + | |iPS152 and iPS151 | ||
| + | |iPS149 and iPS150 | ||
| + | |iPS84 and iPS140 | ||
| + | |- | ||
| + | |Tm | ||
| + | |57,5°C | ||
| + | |56,7°C | ||
| + | |72°C | ||
| + | |- | ||
| + | |t | ||
| + | |1 min 30 | ||
| + | |20 sec | ||
| + | |30 sec | ||
| + | |} | ||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
| + | |||
====Q5 PCR on dCas9 ST - GFP 11 in pSB1C3, FRB in pJET and GFP 1.9 in pUC19 ==== | ====Q5 PCR on dCas9 ST - GFP 11 in pSB1C3, FRB in pJET and GFP 1.9 in pUC19 ==== | ||
Revision as of 12:56, 13 September 2016
Contents
- 1 Wednesday 7th 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 Clean-up of Gibson products
- 1.1.1.3 Transformation of DH5a cells with FRB - GFP 11 in pSB1C3 obtained by Gibson
- 1.1.1.4 Colony PCR of 32 clones containing dCas9 NM - GFP 10 in pSB1C3
- 1.1.1.5 Q5 PCR on dCas9 ST - GFP 11 in pSB1C3, FRB in pJET and GFP 1.9 in pUC19
- 1.1.1.6 NanoDrop Measurements
- 1.1.1.7 Gel of cleaned up PCR products
- 1.1.1 Visualization
- 1.1 Lab work
Wednesday 7th September
Lab work
Visualization
Gibson of cleaned up PCR products FRB from clone 9 x pSB1C3 - GFP 11 from clone 8
By Maxence
Gibson was performed on cleaned up PCR products FRB from clone 9 (insert) x pSB1C3 - GFP 11 from clone 8 (plasmid) with the following protocol:
For each 20μl of reaction, mix the following reagents :
- 0.64 µL of insert
- 3.68 µL of plasmid
- 5.67 µL of water
- 10 µL of buffer
Two controls were done: one without insert and one without buffer (water was added in order to have a total of 20 µL. The PCR was performed as follow : 1 hour at 50°C.
Clean-up of Gibson products
By Maxence
Gibson products obtained were cleaned up by using the NucleoSpin Gel and PCR Clean-up kit protocol.
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 control (no mix added when Gibson performed) using the usual protocol.
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 50μl of reaction, mix the following reagents :
- 1 µL of plasmid
- 1 µL of dNTPs (10mM)
- 1 µL of each primer mix (10µM)
- 10 µL of Q5 buffer (5X)
- 0,5 µL of Q5 high fidelity polymerase
- 35,5 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 | $\infinity\$ |
Primers used were:
| Matrix | dCas9 ST - GFP 11 in pSB1C3 clones 6 and 8 | FRB in pJET clones 4 and 9 | GFP 1.9 in pUC19 |
|---|---|---|---|
| Primers | iPS152 and iPS151 | iPS149 and iPS150 | iPS84 and iPS140 |
| Tm | 57,5°C | 56,7°C | 72°C |
| t | 1 min 30 | 20 sec | 30 sec |
Q5 PCR on dCas9 ST - GFP 11 in pSB1C3, FRB in pJET and GFP 1.9 in pUC19
By Maxence
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)
- 1 µL of each primer mix (10µM)
- 10 µL of Q5 buffer (5X)
- 0,5 µL of Q5 high fidelity polymerase
- 35,5 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 | $\infinity\$ |
Primers used were:
| Matrix | dCas9 ST - GFP 11 in pSB1C3 clones 6 and 8 | FRB in pJET clones 4 and 9 | GFP 1.9 in pUC19 |
|---|---|---|---|
| Primers | iPS152 and iPS151 | iPS149 and iPS150 | iPS84 and iPS140 |
| Tm | 57,5°C | 56,7°C | 72°C |
| t | 1 min 30 | 20 sec | 30 sec |
NanoDrop Measurements
By Maxence
| Sample | Concentration (ng/µL) |
|---|---|
| PCR fragment GFP 11 clone 6 | 187.23 |
| PCR fragment GFP 11 clone 8 | 156.85 |
| PCR fragment FRB clone 4 | 75.67 |
| PCR fragment FRB clone 9 | 246.41 |
| PCR fragment GFP 1.9 | 22.06 |
Gel of cleaned up PCR products
By Maxence
After amplification, 3 µL of each cleaned up 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) |
|---|---|
| GFP 11- pSB1C3 | 2500 |
| FRB | 374 |
| GFP 1.9 | 862 |
GEL GEL GEL
