Team:Lyon-INSA-ENS/Realisation/Week4

From 2011.igem.org

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X + P : 22M, 2L, 24E<br/><br/>
X + P : 22M, 2L, 24E<br/><br/>
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Electrophoresis of the digested plasmids versus the non digested.
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Electrophoresis of the digested plasmids versus the non digested.<br/>
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All the strains had the correct plasmid : they were plated on LB + amp medium.

Revision as of 07:34, 27 July 2011




Week 4


From Monday the 27th of June to Friday the 1st of July 2011







Monday




Tuesday


Culture of NM522 cells for later transformations and Curli for extraction.





Wednesday


Miniprep, digestion and electrophoresis of the Curli plasmid.





Thursday


CaCl2 chemical transformation of some iGEM kit distribution DNA :

Plate 1 :
18A (constitutive promoter, Amp )
2M ( strong RBS, Amp )
5L ( weak RBS, Amp )
22M ( RBS+YFP, Amp)

Plate 2 :
24E (YFP, Amp + Kan )
2L (GFP, Amp )


The local newspaper "VIVA" interviewed us. They ask about our project, our team and about iGEM's organization.





Friday


Miniprep using the QuickPure kit of the previous 6 iGEM parts.

Digestion with :
S + P : 18A, 2M, 5L
X + P : 22M, 2L, 24E

Electrophoresis of the digested plasmids versus the non digested.
All the strains had the correct plasmid : they were plated on LB + amp medium.