Difference between revisions of "Team:Paris Saclay/Notebook/July/21"
m (→Get DNA Closer) |
(→Lab work) |
||
| Line 2: | Line 2: | ||
=Thursday 21<sup>st</sup> July= | =Thursday 21<sup>st</sup> July= | ||
| − | |||
===Biobrick characterization=== | ===Biobrick characterization=== | ||
| Line 9: | Line 8: | ||
We made a digestion of K1372001 plasmid following this [[Team:Paris_Saclay/Experiments#PlasmidDigestion|protocol]]. | We made a digestion of K1372001 plasmid following this [[Team:Paris_Saclay/Experiments#PlasmidDigestion|protocol]]. | ||
| − | We used | + | We used EcoRI and PstI fast digest enzymes. |
After incubation, 3.3 mL of loading dye is added to digestion products. | After incubation, 3.3 mL of loading dye is added to digestion products. | ||
| − | We put | + | We put on gel 10µL of DNA ladder and 20 µL of digestion products. |
We set the eletrophoresis machine at 100V for 25min. | We set the eletrophoresis machine at 100V for 25min. | ||
| Line 32: | Line 31: | ||
A Petri dish with LB and streptomycin was made with: | A Petri dish with LB and streptomycin was made with: | ||
| − | *20 mL of LB agar | + | * 20 mL of LB agar |
| − | *10µL of streptomycin (initial concentration 100mg/mL) | + | * 10µL of streptomycin (initial concentration 100mg/mL) |
| − | + | We added IPTG and xGal on Petri dishes of LB and Ampicillin. | |
| − | We added IPTG and | + | |
For each Petri dish: | For each Petri dish: | ||
| − | *500µL of water | + | * 500µL of water |
| − | *1µL of IPTG | + | * 1µL of IPTG |
| − | *1µL of X-Gal | + | * 1µL of X-Gal |
The solution was spread on Petri dish | The solution was spread on Petri dish | ||
| Line 50: | Line 48: | ||
6 tubes were made. For each tube: | 6 tubes were made. For each tube: | ||
| − | *1 mL LB | + | * 1 mL LB |
| − | *0.5 µL streptomycin | + | * 0.5 µL streptomycin |
The tubes were incubated at 37°C and 180 rpm overnight. | The tubes were incubated at 37°C and 180 rpm overnight. | ||
| Line 61: | Line 59: | ||
DH5α|pPS16_007 that were put in culture the day before showed blue colonies for the clones 5 and 11. Thus those clones can not be used for high fidelity PCR and be sequenced. | DH5α|pPS16_007 that were put in culture the day before showed blue colonies for the clones 5 and 11. Thus those clones can not be used for high fidelity PCR and be sequenced. | ||
| − | A DreamTaq PCR was made with transformed cultures pPS16_002, pPS16_004 and pPS16_007 following the usual [[Team:Paris_Saclay/Experiments#Polymerase_chain_reaction|protocol]] with Tm at 57°C | + | A DreamTaq PCR was made with transformed cultures pPS16_002, pPS16_004 and pPS16_007 following the usual [[Team:Paris_Saclay/Experiments#Polymerase_chain_reaction|protocol]] with Tm at 57°C. |
| − | We divided up the PCR mix in | + | We divided up the PCR mix in 18 PCR tubes and added in each one a different clone from transformed each of our three cultures. |
| − | The picked colonies were | + | The picked colonies were spread on a Petri dish medium LB + Ampicillin (50µg/mL) + X-Gal/IPTG (1/1000). |
Results : | Results : | ||
| Line 80: | Line 78: | ||
|706 | |706 | ||
|} | |} | ||
| − | |||
[[File:T--Paris_Saclay--20160721_PCRpPS16_00247_échelle1.JPG|400px|thumb|right|]] | [[File:T--Paris_Saclay--20160721_PCRpPS16_00247_échelle1.JPG|400px|thumb|right|]] | ||
| − | The electropheresis on agarose gel showed good size product PCR for pPS16_004 | + | The electropheresis on agarose gel showed good size product PCR for pPS16_004 clones 2 to 6, for pPS16_002 clone 5, and pPS16_007 clones 2 and 3. |
{{Team:Paris_Saclay/notebook_footer}} | {{Team:Paris_Saclay/notebook_footer}} | ||
Latest revision as of 15:54, 9 October 2016
