Team:EPF-Lausanne/Notebook/August2011

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(Tuesday, 16 August 2011)
(Tuesday, 16 August 2011)
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Unfortunately the PCR purification gave us bad results for the T7-lysis which is at very low concentration. pSB3C5 instead has an high concentration.
Unfortunately the PCR purification gave us bad results for the T7-lysis which is at very low concentration. pSB3C5 instead has an high concentration.
Henrike suggested, to have an higher yield, to dilute your PCR products 4-fold before starting the PCR purification protocol.
Henrike suggested, to have an higher yield, to dilute your PCR products 4-fold before starting the PCR purification protocol.
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Alessandro will PCR purify the previous succesfully amplified T7-RFP products.
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Alessandro PCR purified the previous succesfully amplified T7-RFP products but for T7-lac-RFP he had a very low yeld so the next day the PCR and purification has to be repeated.
Vincent got the sequences for the Y42F, V36F mutants back. With the help of the BLAST alignment tool, it became clear that the V36F mutant was as expected, while the Y42F was in fact the P39Q-Y42M mutant. It may be that the primers got mixed up or that the labelling of plates was incorrect. Either way, we have two mutants.  
Vincent got the sequences for the Y42F, V36F mutants back. With the help of the BLAST alignment tool, it became clear that the V36F mutant was as expected, while the Y42F was in fact the P39Q-Y42M mutant. It may be that the primers got mixed up or that the labelling of plates was incorrect. Either way, we have two mutants.  

Revision as of 09:21, 17 August 2011