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Team:Paris Saclay/Notebook/July/10
From 2013.igem.org
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:We picked up 2 colonies, seeded them in liquid medium(LB+chloramphenicol), incubation at 37°C, 200rpm during one night.</p><br> | :We picked up 2 colonies, seeded them in liquid medium(LB+chloramphenicol), incubation at 37°C, 200rpm during one night.</p><br> | ||
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| + | {{Team:Paris_Saclay/incl_debut_generique}} | ||
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| + | ='''Notebook : August 23'''= | ||
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| + | =='''Lab work'''== | ||
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| + | ==='''A - Aerobic/Anaerobic regulation system'''=== | ||
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| + | ===='''Objective : obtaining Bba_K1155003, Bba_K1155007'''==== | ||
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| + | ===='''1 - Transformation of Bba_I732019 and Bba_B0010 in DH5α'''==== | ||
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| + | Sheng | ||
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| + | {| | ||
| + | | style="border:1px solid black;padding:5px;background-color:#DE;" | | ||
| + | Transformation of Bba_B0010 of 07/09/13 did work. We will do it again. | ||
| + | |} | ||
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| + | Protocol : [[Team:Paris_Saclay/Protocols/Bacterial transformation|Bacterial transformation]] | ||
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| + | ===='''Objective : obtaining biobricks in PSB3K3'''==== | ||
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| + | ===='''1 - '''==== | ||
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| + | ==='''B - PCB sensor system'''=== | ||
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| + | ===='''Objective : obtaining Bba_K1155001, Bba_K1155002, BphR2 protein'''==== | ||
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| + | ===='''1 - Transformation of ligation of PSB1C3 and BphA1 or BphR1 or BphR2'''==== | ||
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| + | Abdou | ||
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| + | Protocol : [[Team:Paris_Saclay/Protocols/Bacterial transformation|Bacterial transformation]] | ||
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|[[Team:Paris Saclay/Notebook/July/9|<big>Previous day</big>]] | |[[Team:Paris Saclay/Notebook/July/9|<big>Previous day</big>]] | ||
Revision as of 20:45, 23 September 2013
Contents |
Notebook : July 10
Summary:
For regulation system:
- prepared the solution of BioBrick fnr repressor in PsB1C3 plasmid for DNA sequencing.
- the terminator transformation of BBa_B0010 did not work yesterday, a second transformation had been done for it.
- The transformation for RBS+LacZ+terminator plasmid into competent cells was performed.
- after the transformation PSB3K3 plasmid in competent cells, these cells were cultured in a liquid nutritive medium.
For PSBs sensor system:
- the ligation products were transformed into competent cells and were cultured on solid medium with their specific antibiotics.
Lab work
A.aero/anaerobic regulation system:
- BioBrick RBS+LacZ+terminator in plasmid PSB1C3
- BioBrick RBS+amilCP+terminator in plasmid PSB1C3
Transformation
Transformation for BBa_B0010 dit work, we observed 0 colonies on the Petri dish, We decided to redo another transformation
Transformation for BBa_I732019(RBS+LacZ+terminator BBa_B0010):
- the construction of RBS+LacZ+terminator BBa_B0010 is already done and stocked in iGEM BioBrick bank named BBa_I732019 12G p4 kit 2012. So we just suspended the BioBrick with 10µl water, transformed them into 100µl competent cell.
Cloning for plasmid PSB3K3:
- results of transformation and cloning: 34 colonies grown.
- We picked up 2 colonies, seeded them in liquid medium(LB+chloramphenicol), incubation at 37°C, 200rpm during one night.
Notebook : August 23
Lab work
A - Aerobic/Anaerobic regulation system
Objective : obtaining Bba_K1155003, Bba_K1155007
1 - Transformation of Bba_I732019 and Bba_B0010 in DH5α
Sheng
|
Transformation of Bba_B0010 of 07/09/13 did work. We will do it again. |
Protocol : Bacterial transformation
Objective : obtaining biobricks in PSB3K3
1 -
B - PCB sensor system
Objective : obtaining Bba_K1155001, Bba_K1155002, BphR2 protein
1 - Transformation of ligation of PSB1C3 and BphA1 or BphR1 or BphR2
Abdou
Protocol : Bacterial transformation
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