Team:Paris Saclay/Notebook/August/26
From 2013.igem.org
(→lab work) |
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='''Notebook : August 26'''= | ='''Notebook : August 26'''= | ||
- | ==''' | + | =='''Lab work'''== |
- | + | ==='''A - Aerobic/Anaerobic regulation system'''=== | |
- | + | ===='''Objective : characterize BBa_K1155000, BBa_K1155004, BBa_K1155005, BBa_K1155006'''==== | |
- | + | ===='''1 - Digestion of BBa_K1155000, BBa_K1155004, BBa_K1155005, BBa_K1155006 by SpeI/PstI'''==== | |
- | + | ||
- | + | XiaoJing | |
- | + | * BBa_K1155000 : | |
- | * | + | ** DNA : 14µL |
- | ** | + | ** SpeI FD : 2µL |
- | + | ** PstI FD : 2µL | |
- | : | + | ** Buffer FD : 2µL |
- | + | ||
- | : | + | |
- | : | + | * BBa_K1155004 clone 6 : |
+ | ** DNA : 14µL | ||
+ | ** SpeI FD : 2µL | ||
+ | ** PstI FD : 2µL | ||
+ | ** Buffer FD : 2µL | ||
- | + | * BBa_K1155004 clone 7 : | |
- | + | ** DNA : 14µL | |
- | + | ** SpeI FD : 2µL | |
- | + | ** PstI FD : 2µL | |
- | + | ** Buffer FD : 2µL | |
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+ | * BBa_K1155005 clone 6 : | ||
+ | ** DNA : 7µL | ||
+ | ** SpeI FD : 2µL | ||
+ | ** PstI FD : 2µL | ||
+ | ** Buffer FD : 2µL | ||
+ | ** H2O : 7µL | ||
- | + | * BBa_K1155005 clone 7 : | |
+ | ** DNA : 14µL | ||
+ | ** SpeI FD : 2µL | ||
+ | ** PstI FD : 2µL | ||
+ | ** Buffer FD : 2µL | ||
- | + | * BBa_K1155006 clone 6 : | |
- | + | ** DNA : 4µL | |
- | + | ** SpeI FD : 2µL | |
- | + | ** PstI FD : 2µL | |
- | + | ** Buffer FD : 2µL | |
- | + | ** H2O : 10µL | |
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- | : | + | * BBa_K1155004 already digested by SpeI : |
+ | ** DNA : 13µL | ||
+ | ** PstI FD : 2µL | ||
+ | ** Buffer FD : 2µL | ||
+ | ** H2O : 3µL | ||
- | + | * BBa_K1155005 already digested by SpeI : | |
- | + | ** DNA : 10µL | |
- | + | ** PstI FD : 2µL | |
- | + | ** Buffer FD : 2µL | |
- | + | ** H2O : 6µL | |
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- | : | + | * BBa_K1155006 already digested by SpeI : |
+ | ** DNA : 9µL | ||
+ | ** PstI FD : 2µL | ||
+ | ** Buffer FD : 2µL | ||
+ | ** H2O : 7µL | ||
- | + | We incubate the digestion for 30 minutes at 37°C. | |
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- | + | ===='''2 - Inactivation of SpeI/PstI used for the digestion of BBa_K1155000, BBa_K1155004, BBa_K1155005, BBa_K1155006'''==== | |
- | + | ||
- | + | XiaoJing | |
- | + | ||
- | + | Protocol : [[Team:Paris_Saclay/ethanol|Ethanol precipitation]] | |
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- | + | We used 20µL of DNA. | |
- | + | Nanodrop : | |
- | + | * Pndh* : 91.8ng/µL | |
- | + | * NarK clone 6 : 19.8ng/µL | |
- | + | * Nark already digested by SpeI : 15.1ng/µL | |
- | + | * NarG clone 6 : 13.4ng/µL | |
- | + | * NarG clone 7 : 103.9ng/µL | |
- | + | * narG already digested by SpeI : 17.4ng/µL | |
- | + | * NirB clone 6 : 46ng/µL | |
- | + | * NirB clone 7 : 61.6ng/µL | |
- | + | * NirB already digested by SpeI : 16.1ng/µL | |
- | + | ||
- | | | + | {| |
- | + | | style="border:1px solid black;padding:5px;background-color:#DEDEDE;" | | |
- | |- | + | According to the result of the Nanodrop, we decide to do ligations with Pndh* and nirB clone 6. |
- | | | + | |
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|} | |} | ||
+ | ===='''3 - Ligation of Pndh*, NirB clone 6 with RBS-LacZ-Term or RBS-Amil CP-Term in pSB1C3'''==== | ||
+ | XiaoJing | ||
- | + | Used quantities : | |
- | + | NirB clone 6 with RBS-LacZ or RBS-Amil CP, Pndh* with RBS-LacZ or RBS-Amil CP : | |
- | + | * RBS-LacZ-Term or RBS-Amil CP-Term : 3µL | |
- | + | * Pndh* or NirB clone 6 : 5µL | |
- | + | * Buffer ligase : 2µL | |
- | + | * Ligase T4 : 2µL | |
- | + | * H20 : 8µL | |
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- | + | We incubate the ligation for 1h at 37°C. | |
- | + | ===='''4 - Transformation of ligation of Pfnr and NirB with RBS-LacZ-Term or RBS-Amil CP-Term in PSB1C3'''==== | |
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- | + | XiaoJing | |
- | + | Protocol : [[Team:Paris_Saclay/Protocols/Transformation|Bacterial transformation]] | |
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- | : | + | ===='''5- Purification colony from strain MG1655Z1 Δfnr::Km containing plasmid pcp20'''==== |
- | + | XioaJing | |
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- | {| | + | {| |
- | | | + | | style="border:1px solid black;padding:5px;background-color:#DE;" | |
- | + | Transformation of 08/19/13 works. We will purify our colonies. | |
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|} | |} | ||
+ | We streaked colonies into ampicilin and chloramphenicol plates and incubate at 30°C. | ||
+ | ==='''A - Aerobic/Anaerobic regulation system / B - PCB sensor system'''=== | ||
+ | ===='''Objective : obtaining FNR and BphR2'''==== | ||
+ | ===='''1 - Gibson assembly'''==== | ||
- | + | XiaoJing | |
+ | {| | ||
+ | | style="border:1px solid black;padding:5px;background-color:#DE;" | | ||
+ | Tranformation of 08/21 didn't work. We will do the Gibson assembly again. | ||
+ | |} | ||
+ | Used quantities : | ||
- | : | + | * RBS-BphR2 : |
+ | ** PSB1C3 : 3µL | ||
+ | ** BphR2 Part I : 1µL | ||
+ | ** BphR2 Part II : 1µL | ||
+ | ** Gibson mix : 15µL | ||
- | : | + | * FNR : |
+ | ** PSB1C3 : 3µL | ||
+ | ** FNR Part I : 1µL | ||
+ | ** FNR Part II : 1µL | ||
+ | ** Gisbon mix : 15µL | ||
- | + | * RBS-FNR : | |
- | + | ** PSB1C3 : 3µL | |
- | + | ** RBS-FNR Part I : 1µL | |
- | + | ** FNR Part II : 1µL | |
- | + | ** Gibson mix : 15µL | |
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- | + | We keep these mix at 50°C for 1h. | |
- | + | ===='''2 - Transformation of FNR, RBS-FNR and RBS-BphR2 in DH5α'''==== | |
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+ | XiaoJing | ||
- | + | Protocol : [[Team:Paris_Saclay/Protocols/Transformation|Bacterial transformation]] | |
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{| border="1" align="center" | {| border="1" align="center" | ||
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|[[Team:Paris_Saclay/Notebook|<big>Back to calendar</big>]] | |[[Team:Paris_Saclay/Notebook|<big>Back to calendar</big>]] | ||
- | |[[Team:Paris Saclay/Notebook/ | + | |[[Team:Paris Saclay/Notebook/August/27|<big>Next day</big>]] |
|} | |} | ||
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{{Team:Paris_Saclay/incl_fin}} | {{Team:Paris_Saclay/incl_fin}} |
Latest revision as of 22:16, 4 October 2013
Notebook : August 26
Lab work
A - Aerobic/Anaerobic regulation system
Objective : characterize BBa_K1155000, BBa_K1155004, BBa_K1155005, BBa_K1155006
1 - Digestion of BBa_K1155000, BBa_K1155004, BBa_K1155005, BBa_K1155006 by SpeI/PstI
XiaoJing
- BBa_K1155000 :
- DNA : 14µL
- SpeI FD : 2µL
- PstI FD : 2µL
- Buffer FD : 2µL
- BBa_K1155004 clone 6 :
- DNA : 14µL
- SpeI FD : 2µL
- PstI FD : 2µL
- Buffer FD : 2µL
- BBa_K1155004 clone 7 :
- DNA : 14µL
- SpeI FD : 2µL
- PstI FD : 2µL
- Buffer FD : 2µL
- BBa_K1155005 clone 6 :
- DNA : 7µL
- SpeI FD : 2µL
- PstI FD : 2µL
- Buffer FD : 2µL
- H2O : 7µL
- BBa_K1155005 clone 7 :
- DNA : 14µL
- SpeI FD : 2µL
- PstI FD : 2µL
- Buffer FD : 2µL
- BBa_K1155006 clone 6 :
- DNA : 4µL
- SpeI FD : 2µL
- PstI FD : 2µL
- Buffer FD : 2µL
- H2O : 10µL
- BBa_K1155004 already digested by SpeI :
- DNA : 13µL
- PstI FD : 2µL
- Buffer FD : 2µL
- H2O : 3µL
- BBa_K1155005 already digested by SpeI :
- DNA : 10µL
- PstI FD : 2µL
- Buffer FD : 2µL
- H2O : 6µL
- BBa_K1155006 already digested by SpeI :
- DNA : 9µL
- PstI FD : 2µL
- Buffer FD : 2µL
- H2O : 7µL
We incubate the digestion for 30 minutes at 37°C.
2 - Inactivation of SpeI/PstI used for the digestion of BBa_K1155000, BBa_K1155004, BBa_K1155005, BBa_K1155006
XiaoJing
Protocol : Ethanol precipitation
We used 20µL of DNA.
Nanodrop :
- Pndh* : 91.8ng/µL
- NarK clone 6 : 19.8ng/µL
- Nark already digested by SpeI : 15.1ng/µL
- NarG clone 6 : 13.4ng/µL
- NarG clone 7 : 103.9ng/µL
- narG already digested by SpeI : 17.4ng/µL
- NirB clone 6 : 46ng/µL
- NirB clone 7 : 61.6ng/µL
- NirB already digested by SpeI : 16.1ng/µL
According to the result of the Nanodrop, we decide to do ligations with Pndh* and nirB clone 6. |
3 - Ligation of Pndh*, NirB clone 6 with RBS-LacZ-Term or RBS-Amil CP-Term in pSB1C3
XiaoJing
Used quantities :
NirB clone 6 with RBS-LacZ or RBS-Amil CP, Pndh* with RBS-LacZ or RBS-Amil CP :
- RBS-LacZ-Term or RBS-Amil CP-Term : 3µL
- Pndh* or NirB clone 6 : 5µL
- Buffer ligase : 2µL
- Ligase T4 : 2µL
- H20 : 8µL
We incubate the ligation for 1h at 37°C.
4 - Transformation of ligation of Pfnr and NirB with RBS-LacZ-Term or RBS-Amil CP-Term in PSB1C3
XiaoJing
Protocol : Bacterial transformation
5- Purification colony from strain MG1655Z1 Δfnr::Km containing plasmid pcp20
XioaJing
Transformation of 08/19/13 works. We will purify our colonies. |
We streaked colonies into ampicilin and chloramphenicol plates and incubate at 30°C.
A - Aerobic/Anaerobic regulation system / B - PCB sensor system
Objective : obtaining FNR and BphR2
1 - Gibson assembly
XiaoJing
Tranformation of 08/21 didn't work. We will do the Gibson assembly again. |
Used quantities :
- RBS-BphR2 :
- PSB1C3 : 3µL
- BphR2 Part I : 1µL
- BphR2 Part II : 1µL
- Gibson mix : 15µL
- FNR :
- PSB1C3 : 3µL
- FNR Part I : 1µL
- FNR Part II : 1µL
- Gisbon mix : 15µL
- RBS-FNR :
- PSB1C3 : 3µL
- RBS-FNR Part I : 1µL
- FNR Part II : 1µL
- Gibson mix : 15µL
We keep these mix at 50°C for 1h.
2 - Transformation of FNR, RBS-FNR and RBS-BphR2 in DH5α
XiaoJing
Protocol : Bacterial transformation
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