Team:EPF-Lausanne/Notebook/August2011

From 2011.igem.org

(Difference between revisions)
(Tuesday, 16 August 2011)
(Tuesday, 16 August 2011)
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Nadine got the sequencing results for digested-ligated pSB3K1 Pconst-TetR and they look fine! There is no trace of RFP, and Pconst-TetR are perfect. Seems that we have our 1st beer award.
Nadine got the sequencing results for digested-ligated pSB3K1 Pconst-TetR and they look fine! There is no trace of RFP, and Pconst-TetR are perfect. Seems that we have our 1st beer award.
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Alessandro ran the gel for the PCR products of the previous day: we miss pSB3K1 therefore the reaction has been repeated with different templates (even with the plasmid from the registry). Another PCR has been run to amplify the backbone from pSB3K5.
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Alessandro ran the gel for the PCR products of the previous day: we miss pSB3K1 therefore the reaction has been repeated with different templates (even with the plasmid from the registry) and it worked. Another PCR has been run to amplify the backbone from pSB3K5 but it didn't work (maybe because the plasmid taken from the registry's plate has a very low concentration); the reaction will be repeated only after the miniprep for this sample will be done.
Alessandro proceeded with the protocol started the day before from Henrike to make competent cells: the BL21 (DE3) which will be used for the T7-lys plasmid since these bacteria have the T7 polymerase gene under the control of Plac (they overexpress LacI).
Alessandro proceeded with the protocol started the day before from Henrike to make competent cells: the BL21 (DE3) which will be used for the T7-lys plasmid since these bacteria have the T7 polymerase gene under the control of Plac (they overexpress LacI).
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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.
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Revision as of 14:15, 16 August 2011