EPF-Lausanne/28 August 2009
From 2009.igem.org
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(→Characterisation of RO2 + LacI-RBS) |
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We used the reader in Sebastian's lab (qPCR machine). | We used the reader in Sebastian's lab (qPCR machine). | ||
- | We took 3 clones of RO2 (3 in M9, 3 in LB), and put 50 ul in each well. In 3 wells we add ATC ( | + | We took 3 clones of RO2 (3 in M9, 3 in LB), and put 50 ul in each well. In 3 wells we add ATC (5 ul), in 3 other nothing, in the next 3 TRP (5 ul) and finally in the last 3 IPTG (5 ul, to induce LacI). |
+ | |||
+ | It was put for 2 hours at 37°C and 1 picture was taken each 3 minutes. | ||
+ | |||
+ | The '''results''' weren't concluding : | ||
+ | |||
+ | - All clones with ATC (no matter M9 or LB) had a "linear" progression. | ||
+ | |||
+ | - The clones (M9 and LB) with nothing and TRP didn't make any difference (linear half way then growing a little bit exponentially). | ||
+ | |||
+ | - LacI-RBS-GFP clones didn't seem to react to the IPTG induction (same pattern as those which hadn't been induced). | ||
+ | |||
+ | '''Analysis of the results''' | ||
==People in the lab== | ==People in the lab== |
Revision as of 10:08, 4 September 2009
Wet Lab
We did a glycerol stock out of the 3 LR2+GFP clones : LacI-RBS #1, #2 #4 + GFP (E02110).
Characterisation of RO2 + LacI-RBS
We used the reader in Sebastian's lab (qPCR machine).
We took 3 clones of RO2 (3 in M9, 3 in LB), and put 50 ul in each well. In 3 wells we add ATC (5 ul), in 3 other nothing, in the next 3 TRP (5 ul) and finally in the last 3 IPTG (5 ul, to induce LacI).
It was put for 2 hours at 37°C and 1 picture was taken each 3 minutes.
The results weren't concluding :
- All clones with ATC (no matter M9 or LB) had a "linear" progression.
- The clones (M9 and LB) with nothing and TRP didn't make any difference (linear half way then growing a little bit exponentially).
- LacI-RBS-GFP clones didn't seem to react to the IPTG induction (same pattern as those which hadn't been induced).
Analysis of the results
People in the lab
Basile, Rafael, Nicolas