(→PCR of DH5αlpPS16_008 with Dream Taq and electrophoresis) |
(→Lab work) |
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{{Team:Paris_Saclay/notebook_header}} | {{Team:Paris_Saclay/notebook_header}} | ||
=Wednesday 13<sup>th</sup> July= | =Wednesday 13<sup>th</sup> July= | ||
− | |||
===Bringing DNA closer=== | ===Bringing DNA closer=== | ||
− | ====Glycerol stocks | + | ====Glycerol stocks of DH5α transformed with DS-NMcas, DS-SPcasN-, DS-ST1casN- and DS-TDcasN-==== |
''By Laetitia'' | ''By Laetitia'' | ||
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* Cl1 and Cl2 of DS-ST1casN- | * Cl1 and Cl2 of DS-ST1casN- | ||
* Cl1 and Cl2 of DS-TDcasN- | * Cl1 and Cl2 of DS-TDcasN- | ||
− | |||
For 1 glycerol stock: | For 1 glycerol stock: | ||
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''By Caroline'' | ''By Caroline'' | ||
− | The different parts needed | + | The different parts needed to the bring DNA closer tool were amplified by high fidelity PCR using Phusion following [[Team:Paris_Saclay/Experiments#phusionPCR|usual protocol]] with a TM at 60°C. [[Team:Paris_Saclay/Experiments#primers|Specific primers]] for these constructs were used to amplify. These primers will allow the Gibson assembly afterward : Ptet_R and Ptet_F for the plasmids, Link-TDdcas_F and Ter_TDdcas_R for DS_TDcasN, Tet-SPdcas_F and Link-SPdcas_R for DS_SPcasN. |
===Biobrick characterization=== | ===Biobrick characterization=== | ||
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''By Mathilde and Charlène'' | ''By Mathilde and Charlène'' | ||
− | We did an [[Team:Paris_Saclay/Experiments#ElectroCompetent| | + | We did an [[Team:Paris_Saclay/Experiments#ElectroCompetent|electrotransformation]] of BL21 with : |
* pcl_TAA + K1372001 (time constant equal to 5.9ms) | * pcl_TAA + K1372001 (time constant equal to 5.9ms) | ||
* pcl_TAG + K1372001 (time constant equal to 6 ms) | * pcl_TAG + K1372001 (time constant equal to 6 ms) | ||
* pcl_Tq + K1372001 (time constant equal to 6 ms) | * pcl_Tq + K1372001 (time constant equal to 6 ms) | ||
− | Cells were | + | Cells were spread on LB + Streptomycin (50µg/mL) + Chloramphenicol (30µg/mL) medium. For each condition, we made a Petri dish with 50µL of cells and another with 500µL of cells. |
===Visualization=== | ===Visualization=== | ||
− | ====PCR of | + | ====PCR of DH5$\alpha$α|pPS16_008 with Dream Taq and electrophoresis ==== |
''By Laetitia '' | ''By Laetitia '' | ||
Preparation of the PCR mix (total of 200μL ): | Preparation of the PCR mix (total of 200μL ): | ||
− | *20 μL of Dream Taq Green Buffer | + | * 20 μL of Dream Taq Green Buffer |
− | *20 μL of dNTP (10 mM) | + | * 20 μL of dNTP (10 mM) |
− | *8 μL of primer 1151 (10 mM) | + | * 8 μL of primer 1151 (10 mM) |
− | *8 μL of primer 1152 (10 mM) | + | * 8 μL of primer 1152 (10 mM) |
− | *1,04 μL of Dream Taq | + | * 1,04 μL of Dream Taq |
− | *142,96 μL of Nuclease free water | + | * 142,96 μL of Nuclease free water |
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We picked 1 white clone in the petri dish containing DH5αlpPS16_008 (from 12/07/16) and soaked it in the tube (with PCR mix) | We picked 1 white clone in the petri dish containing DH5αlpPS16_008 (from 12/07/16) and soaked it in the tube (with PCR mix) | ||
− | + | PCR was performed using [[Team:Paris_Saclay/Experiments#Polymerase_chain_reaction|this program]] : | |
− | + | We used a TM at 57°C. | |
− | + | The products from the PCR were migrated on gel by electrophoresis during 20 min. We used the blue scale. | |
− | ====Culture of | + | ====Culture of DH5α|[[Team:Paris_Saclay/Notebook/June/28#pPS16_008|pPS16_008 clones]] on petri dish==== |
''By Laetitia '' | ''By Laetitia '' | ||
− | We divided a Petri dish in 7(for 7 clones from DH5αlpPS16_008). | + | We divided a Petri dish in 7 (for 7 clones from DH5αlpPS16_008). |
− | Just after putting the DH5αlpPS16_008 clone in the PCR tube, spread the cells with the stick on the part corresponding to the clone on the petri dish. | + | Just after putting the DH5αlpPS16_008 clone in the PCR tube, we spread the cells with the stick on the part corresponding to the clone on the petri dish. |
We left it grow at room temperature. | We left it grow at room temperature. | ||
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''By Alice'' | ''By Alice'' | ||
− | High fidelity PCR perfomed on the [[Team:Paris_Saclay/Notebook/July/12#Q5 PCR pPS16_004 and pPS16_007|12/07/16]] did not give expected results. Thus high fidelity colony PCR is performed again on bacteria transformed with pPS16_007 following [[Team:Paris_Saclay/Experiments#Q5PCR|this protocol]]. [[Team:Paris_Saclay/Experiments#primers|1151_pheoR and 1152_pheoF]] primers were used. Annealing temperature was 60°C. After amplification, 1 µL of loading dye was added to 5µL of each PCR products. Then 5 µL of this mix were put | + | High fidelity PCR perfomed on the [[Team:Paris_Saclay/Notebook/July/12#Q5 PCR pPS16_004 and pPS16_007|12/07/16]] did not give expected results. Thus high fidelity colony PCR is performed again on bacteria transformed with pPS16_007 following [[Team:Paris_Saclay/Experiments#Q5PCR|this protocol]]. [[Team:Paris_Saclay/Experiments#primers|1151_pheoR and 1152_pheoF]] primers were used. Annealing temperature was 60°C. After amplification, 1 µL of loading dye was added to 5µL of each PCR products. Then 5 µL of this mix were put on gel. PCR products were migrated 30min at 100V. |
PCR products expected were : | PCR products expected were : | ||
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====Colony screening PCR on bacteria transformed with [[Team:Paris_Saclay/Notebook/July/4#pPS16_004|pPS16_004]]==== | ====Colony screening PCR on bacteria transformed with [[Team:Paris_Saclay/Notebook/July/4#pPS16_004|pPS16_004]]==== | ||
''By Alice and Caroline'' | ''By Alice and Caroline'' | ||
+ | <div id="PCRcolony_2.2_4.1"></div> | ||
− | Clones of bacteria transformed with pPS16_004 selected on the [[Team:Paris_Saclay/Notebook/July/11#Colony screening PCR pPS16_004 and pPS16_007|11/07/16]] did not grow on petri dishes. That why we performed again colony screening PCR on these bacteria. After transformation, only white bacteria were selected (blue white screen) | + | Clones of bacteria transformed with pPS16_004 selected on the [[Team:Paris_Saclay/Notebook/July/11#Colony screening PCR pPS16_004 and pPS16_007|11/07/16]] did not grow on petri dishes. That why we performed again colony screening PCR on these bacteria. After transformation, only white bacteria were selected (blue/white screen). PCR with DreamTaq Polymerase was performed following [[Team:Paris_Saclay/Experiments#taqPCR|this protocol]]. Clones selected for PCR were kept on LB+Amp+XGal(2µLXGal/1000µLH2O)+IPTG(2µLIPTG/1000µLH2O). Two primers ([[Team:Paris_Saclay/Experiments#primers|1151_pheoR and 1152_pheoF]]) were used. Annealing temperature was 53°C. After amplification, 5 µL of each PCR products and 10 µL of DNA ladder were placed on gel and migrated at 100v during 30 min. |
PCR products expected were: | PCR products expected were: | ||
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|} | |} | ||
+ | No PCR products were observed, despite the experiment was performed twice. | ||
{{Team:Paris_Saclay/notebook_footer}} | {{Team:Paris_Saclay/notebook_footer}} |
Latest revision as of 15:31, 9 October 2016