Team:EPF-Lausanne/Notebook/August2011

From 2011.igem.org

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(Wednesday, 24 August 2011)
 
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Clearly the RFP T7 promoter variants went well, but the T7 Lysis promoter variants ... not so much. Vincent made liquid cultures of all the T7 lysis plasmids (both C5 and K1) and put them in the incubator. He also pelleted all the C5 RFP liquid cultures and the K1-Lys cultures that he had made on Monday (6 colonies per promoter) thinking that he had not yet achieved a full T7-lysis. The pellets are being kept in a special box called "Pellets".
Clearly the RFP T7 promoter variants went well, but the T7 Lysis promoter variants ... not so much. Vincent made liquid cultures of all the T7 lysis plasmids (both C5 and K1) and put them in the incubator. He also pelleted all the C5 RFP liquid cultures and the K1-Lys cultures that he had made on Monday (6 colonies per promoter) thinking that he had not yet achieved a full T7-lysis. The pellets are being kept in a special box called "Pellets".
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Lilia made linear templates out of the mutants plasmids, here the T7 promoter was added to be able to use it for in vitro translation/transcription with the TNT T7 ITT wheat germ extract kit.
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[[File:EPFL2011_muTetRs_linear_template_PCRresults.png|350px]]
== Wednesday, 24 August 2011 ==
== Wednesday, 24 August 2011 ==
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[[File:T7lysis_variants.jpg|600px]]
[[File:T7lysis_variants.jpg|600px]]
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Apparently, 14 through 17 were amplified correctly.  
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Apparently, 14 through 17 were amplified correctly.
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Lilia made a PCR with the primers containing biobrick extentions (prefix and sufix) on the linear templates of the muTetRs.  
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[[File:EPFL2011_muTetRs_1st_biobrick_PCR_on_linear_template.png|350px]]
== Thursday, 25 August 2011 ==
== Thursday, 25 August 2011 ==

Latest revision as of 09:04, 21 September 2011