EPF-Lausanne/7 July 2009
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+ | <font size="6" color="#007CBC"><i>7 July 2009</i></font> | ||
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+ | <br> | ||
+ | ---- | ||
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+ | ==Wet Lab== | ||
We have to grow the 3 strains generously sent by [mailto:j.beatty@ubc.ca Tom Beatty] | We have to grow the 3 strains generously sent by [mailto:j.beatty@ubc.ca Tom Beatty] | ||
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- | + | ==Cloning Strategy== | |
To design plasmids : software Vector NTI | To design plasmids : software Vector NTI | ||
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+ | ==People in the lab== | ||
+ | :Tu, Heidi, Rafael, Basile, Nath | ||
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+ | <a href="https://2009.igem.org/EPF-Lausanne/8_July_2009"><img src="https://static.igem.org/mediawiki/2009/thumb/5/5e/Fleche_droite.png/70px-Fleche_droite.png"></a></center></html> | ||
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Latest revision as of 08:49, 28 July 2009
Wet Lab
We have to grow the 3 strains generously sent by Tom Beatty
The three strains are :
- R.Palustris CEA001 (wild type) ; should be grown on LB medium only
- R.Palustris BPHP1+ ; should be grown on LB with gentamycin (100 micrograms/ml)
- E.Coli DH10B (pBPH/hmu0) ; should be grown on LB with gentamycin (20 micorgrams/ml)
The transformed LOVTAP and TrpR worked well (N.B. the plasmid of TrpR is pUC19 so the antibiotic resistance is Amp -> see below)
We did the glycerol stock, located in the -80 fridge, first floor of the iGEM compartement.
Then, a miniprep was done with both cultures. A LOVTAP plasmid aliquot was done, a TrpR plasmid aliquot was done, located in the -20 fridge, 2nd floor.
Cloning Strategy
To design plasmids : software Vector NTI
People in the lab
- Tu, Heidi, Rafael, Basile, Nath