Team:Paris Saclay/Notebook/July/3
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- | + | ='''Notebook : July 3'''= | |
- | + | =='''Lab work'''== | |
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- | + | ==='''A - Aerobic/Anaerobic regulation system'''=== | |
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+ | ===='''Objective : obtaining BBa_K1155000'''==== | ||
+ | ===='''1 - Colony PCR of BBa_K1155000 to check good insertion of Pndh* in pSB1C3'''==== | ||
+ | Abdou, Sheng, Zhou | ||
+ | {| | ||
+ | | style="border:1px solid black;padding:5px;background-color:#DE;" | | ||
+ | Tranformation of 07/02/13 works. We will do a PCR colony. | ||
+ | |} | ||
+ | Colonies count for BBa_K1155000 : | ||
+ | * Standard concentration : | ||
+ | ** BBa_K1155000 : 0 colony | ||
+ | * High concentration : | ||
+ | ** BBa_K1155000 : 2 colonies | ||
+ | [[File:Ps0307jour.jpg|300px]] | ||
+ | <br> | ||
+ | <center>[[File:PSprimer07.jpg|right|250px]]</center> | ||
+ | <br> | ||
+ | '''[https://2013.igem.org/Team:Paris_Saclay/Primers Primers] and PCR :''' | ||
+ | <p>'''VF2, VR, Pfnr_up, Pfnr_down are four oligos that we used for plasmid amplification. We used tree combinaisons VF/VR, VF/Pfnr_Down, Pfnr_Up/VR.''' | ||
+ | '''If the promoter Pndh* insert pSB1C3 plasmid successfully, tree fragments with specific size will be amplified.''' </p> | ||
+ | ''' | ||
+ | Protocol''' | ||
- | + | We resuspend each colony with 20µL of H2O. | |
- | + | Used quantities : | |
+ | * DNA : 2µL | ||
+ | * Mix : (it was divided in tubes for 4 different colonies for each oligo combinaison with 23µL of mix in each tube) | ||
+ | ** VF or Pfnr_Up : 6µL | ||
+ | ** VR or Pfnr_Down : 6µL | ||
+ | ** dNTP 10mM : 6µL | ||
+ | ** Buffer Dream Taq : 30µL | ||
+ | ** Dream Taq : 6µL | ||
+ | ** H2O : 246µL | ||
- | + | [[File:PSPCR0307.jpg|400px]] | |
- | ===''' | + | ===='''2 - Culture of BBa_K1155000 '''==== |
- | + | Sheng | |
- | + | We made new cultures by streaking 2 colonies of 07/02/13 culture of BBa_K1155000. We also did liquid culture of each one. | |
+ | We incubate culture at 37°C. | ||
- | + | ===='''Objective : obtaining BBa_K1155003, BBa_K1155007'''==== | |
+ | |||
+ | ===='''1 - Culture of BBa_I732017, BBa_K592009 '''==== | ||
+ | |||
+ | Sheng | ||
{| | {| | ||
| style="border:1px solid black;padding:5px;background-color:#DE;" | | | style="border:1px solid black;padding:5px;background-color:#DE;" | | ||
- | Tranformation of 07/02/13 works. We will do | + | Tranformation of 07/02/13 works. We will do new cultures. |
|} | |} | ||
- | + | We made new cultures by streaking 2 colonies of 07/02/13 culture of BBa_I732017, BBa_K592009. We also did liquid culture of each one. | |
- | + | We incubate culture at 37°C. | |
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Latest revision as of 00:51, 5 October 2013
Contents |
Notebook : July 3
Lab work
A - Aerobic/Anaerobic regulation system
Objective : obtaining BBa_K1155000
1 - Colony PCR of BBa_K1155000 to check good insertion of Pndh* in pSB1C3
Abdou, Sheng, Zhou
Tranformation of 07/02/13 works. We will do a PCR colony. |
Colonies count for BBa_K1155000 :
- Standard concentration :
- BBa_K1155000 : 0 colony
- High concentration :
- BBa_K1155000 : 2 colonies
Primers and PCR :
VF2, VR, Pfnr_up, Pfnr_down are four oligos that we used for plasmid amplification. We used tree combinaisons VF/VR, VF/Pfnr_Down, Pfnr_Up/VR. If the promoter Pndh* insert pSB1C3 plasmid successfully, tree fragments with specific size will be amplified.
Protocol
We resuspend each colony with 20µL of H2O.
Used quantities :
- DNA : 2µL
- Mix : (it was divided in tubes for 4 different colonies for each oligo combinaison with 23µL of mix in each tube)
- VF or Pfnr_Up : 6µL
- VR or Pfnr_Down : 6µL
- dNTP 10mM : 6µL
- Buffer Dream Taq : 30µL
- Dream Taq : 6µL
- H2O : 246µL
2 - Culture of BBa_K1155000
Sheng
We made new cultures by streaking 2 colonies of 07/02/13 culture of BBa_K1155000. We also did liquid culture of each one. We incubate culture at 37°C.
Objective : obtaining BBa_K1155003, BBa_K1155007
1 - Culture of BBa_I732017, BBa_K592009
Sheng
Tranformation of 07/02/13 works. We will do new cultures. |
We made new cultures by streaking 2 colonies of 07/02/13 culture of BBa_I732017, BBa_K592009. We also did liquid culture of each one. We incubate culture at 37°C.
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