Team:Paris Saclay/Notebook/September/3
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+ | {{Team:Paris_Saclay/notebook_header}} | ||
+ | =Wednesday 3rd September= | ||
+ | |||
==LabWork== | ==LabWork== | ||
- | === | + | ===Construction of the fusion protein=== |
We made a classic exttraction of plasmids from the liquid cultures. | We made a classic exttraction of plasmids from the liquid cultures. | ||
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- | === | + | ===Lemon scent=== |
''by Mélanie'' | ''by Mélanie'' | ||
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Electrophoresis of the PCR made [https://2014.igem.org/Team:Paris_Saclay/Notebook/September/2#Limonene_synthase_PCR Yesterday] | Electrophoresis of the PCR made [https://2014.igem.org/Team:Paris_Saclay/Notebook/September/2#Limonene_synthase_PCR Yesterday] | ||
- | [ | + | [[File:0309 PCR LS + extraction pPS5.jpg|400px|center]] |
+ | |||
+ | well 2-3 = PCR with Dream taq or Vent taq | ||
+ | |||
+ | (well 4-5 = checking of the pps5 Extraction) | ||
+ | |||
The PCR have success so I use the PCR clean up kit to purify it | The PCR have success so I use the PCR clean up kit to purify it | ||
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Electrophoresis after purification | Electrophoresis after purification | ||
- | [[File:0309 | + | [[File:0309 purif LS.jpg|400px|center]] |
- | |||
- | + | ====Digestion==== | |
+ | In order to clone LS in pPSI, i Digest it by PacI | ||
+ | |||
+ | {| class="wikitable centre" width="50%" | ||
+ | |+ | ||
+ | |- | ||
+ | ! scope=col | component | ||
+ | ! scope=col | volume | ||
+ | |- | ||
+ | |H<sub>2</sub>O | ||
+ | |3μl | ||
+ | |- | ||
+ | |buffer | ||
+ | |1μl | ||
+ | |- | ||
+ | |PacI | ||
+ | |1μl | ||
+ | |- | ||
+ | |PCR purify | ||
+ | |5μl | ||
+ | |} | ||
====Ligation==== | ====Ligation==== | ||
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Electrophoresis | Electrophoresis | ||
- | [[File:0309 digestion SalI pPS5.jpg|500px]] | + | [[File:0309 digestion SalI pPS5.jpg|500px|center]] |
We saw that we have something strang with our plasmid but we wil check it tomorrow with a good ladder (the ladder here was normally on the well 1) | We saw that we have something strang with our plasmid but we wil check it tomorrow with a good ladder (the ladder here was normally on the well 1) | ||
- | ===pPS3 and pPS4=== | + | ====pPS3 and pPS4==== |
We digest the plasmid by HindIII to direct our insert | We digest the plasmid by HindIII to direct our insert | ||
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|} | |} | ||
- | [[File:0309 digestion HindIII pPS3 4.jpg|500px]] | + | [[File:0309 digestion HindIII pPS3 4.jpg|500px|center]] |
well 1 = ladder | well 1 = ladder | ||
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results are very strange | results are very strange | ||
+ | |||
+ | ==Photo of the Day== | ||
+ | [[File:Paris Saclay 3_september.jpg|250px|center]] | ||
+ | |||
+ | [http://iramis.cea.fr/llb/Phocea/Pisp/visu.php?id=35&uid=%20alexei.grinbaum Alexei Grinbaum] , one of those few we have interviewed during this month of september. | ||
+ | |||
+ | To learn more about the ethic aspect of our project, just click [https://2014.igem.org/Team:Paris_Saclay/Ethics here] | ||
+ | |||
+ | |||
+ | {{Team:Paris_Saclay/notebook_footer}} |
Latest revision as of 12:50, 14 October 2014
Contents |
Wednesday 3rd September
LabWork
Construction of the fusion protein
We made a classic exttraction of plasmids from the liquid cultures.
Check by electrophoresis if it worked and send it for sequencing.
Lemon scent
by Mélanie
PCR LS
Electrophoresis of the PCR made Yesterday
well 2-3 = PCR with Dream taq or Vent taq
(well 4-5 = checking of the pps5 Extraction)
The PCR have success so I use the PCR clean up kit to purify it
Electrophoresis after purification
Digestion
In order to clone LS in pPSI, i Digest it by PacI
component | volume |
---|---|
H2O | 3μl |
buffer | 1μl |
PacI | 1μl |
PCR purify | 5μl |
Ligation
We already have some pPSI digested and dephosphorelated
So I do a ligation:
component | volume |
---|---|
H2O | 5μl |
buffer | 2μl |
ligase | 1μl |
pPSI | 2μl |
LS PCR | 10μl |
2 hours at room temperature and over night at 4°
pPS5
Plasmid exctraction using the kit (picture is here)
digestion by SalI
component | volume |
---|---|
H2O | 11μl |
buffer | 5μl |
SalI | 2μl |
pPS5 | 30μl |
Electrophoresis
We saw that we have something strang with our plasmid but we wil check it tomorrow with a good ladder (the ladder here was normally on the well 1)
pPS3 and pPS4
We digest the plasmid by HindIII to direct our insert
component | volume |
---|---|
H2O | 6μl |
buffer | 1μl |
HindIII | 1μl |
pPS3/4 | 2μl |
well 1 = ladder well 2-3-4 = pPS3 Well 5-6-7 = pPS4
results are very strange
Photo of the Day
[http://iramis.cea.fr/llb/Phocea/Pisp/visu.php?id=35&uid=%20alexei.grinbaum Alexei Grinbaum] , one of those few we have interviewed during this month of september.
To learn more about the ethic aspect of our project, just click here