Team:EPF-Lausanne/Notebook/July2011

From 2011.igem.org

(Difference between revisions)
(Tuesday, 02 August 2011)
 
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The Mutation PCR yielded no product, probably because the primers were too diluted. It has been repeated with a higher primer concentration.
The Mutation PCR yielded no product, probably because the primers were too diluted. It has been repeated with a higher primer concentration.
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== Tuesday, 02 August 2011 ==
 
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Lilia came on Saturday to take the plates and here are the results:
 
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[[File:EPFL2011_plates_020811.png|600px]]
 
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[[File:EPFL2011_Plate020811.png|600px]]
 
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The old competents cells seem not to work very well and the Gibson assembly failed since in the plate with only backbone we have a lot of cells therefore the backbone can closes on itself.
 
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Alessandro make the PCR (gradient PCR in which the annealing temperature increases for each sample) to amplify TetR (putting Pconst in front of it) from Repressilator plasmid to make the Gibson for the Pconst-TetR plasmid.
 
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The result is this:
 
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[[File:EPFL2011_Pcr_02_08.jpg|thumb|200px|Gradient PCR shows a band of the expected size (725 bp)]]
 
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Since we have already amplified the backbone (pSB3K1) we can make the Gibson assembly to make the Pconst-TetR plasmid.
 
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Latest revision as of 16:18, 2 August 2011