1L of agarose gel TAE 0,5X agarose 0,8% was prepared following the usual [[Team:Paris_Saclay/Experiments#DNA_electrophoresis_on_agarose_gel│protocol]]
+
1L of agarose gel TAE 0,5X agarose 0,8% was prepared following the usual [[Team:Paris_Saclay/Experiments#DNA_electrophoresis_on_agarose_gel|protocol]]
Line 13:
Line 13:
Primers IPS 134 and IPS 135 were used to amplify TD-CAS9, NM-cas9 and ST1-cas9. Primers SP1 (IPS 134 + IPS 136) and SP2 (IPS 137 + IPS 135) were used for DS-SPCasN- .
Primers IPS 134 and IPS 135 were used to amplify TD-CAS9, NM-cas9 and ST1-cas9. Primers SP1 (IPS 134 + IPS 136) and SP2 (IPS 137 + IPS 135) were used for DS-SPCasN- .
Primers were diluted in order to get a 100µM final concentration.
Primers were diluted in order to get a 100µM final concentration.
−
The usual [[Team:Paris_Saclay/Experiments#Polymerase_chain_reaction│protocol]] for polymerase q5 PCR was followed, with a Tm=65°c.
+
The usual [[Team:Paris_Saclay/Experiments#Polymerase_chain_reaction|protocol]] for polymerase q5 PCR was followed, with a Tm=65°c.
====PZA21 q5 high fidelity PCR ====
====PZA21 q5 high fidelity PCR ====
Line 19:
Line 19:
PZA21 plasmids were amplified with primers:
PZA21 plasmids were amplified with primers:
−
• Ter_SPdcas_R and Link-SPdcas_R
+
* Ter_SPdcas_R and Link-SPdcas_R
−
• Link-TDdcas_F and Ter_TDdcas_R
+
* Link-TDdcas_F and Ter_TDdcas_R
−
• Ptet R and Ptet F
+
* Ptet R and Ptet F
+
Primers stocks (100µM) were diluted as follows:
Primers stocks (100µM) were diluted as follows:
−
• Add 280µL of H2O nuclease free to Ter_SPdcas_R and 558 µL to Link-SPdcas_R
+
* Add 280µL of H2O nuclease free to Ter_SPdcas_R and 558 µL to Link-SPdcas_R
−
• Add 599µL of H2O nuclease free to Link-TDdcas_F and 219µL to Ter_TDdcas_R
+
* Add 599µL of H2O nuclease free to Link-TDdcas_F and 219µL to Ter_TDdcas_R
−
• Add 191µL of H2O nuclease free to Ptet F and 315µL to Ptet R.
+
* Add 191µL of H2O nuclease free to Ptet F and 315µL to Ptet R.
