Team:EPF-Lausanne/Notebook/August2011

From 2011.igem.org

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(Thursday, 25 August 2011)
(Friday, 26 August)
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In order to continue with the production of T7 promoter variants, Vincent had to make more gene-specific Lysis (i.e. T4 Lysis with RBS upstream). For this, Vincent used the new Hifi+ enzyme that had been ordered the previous day. Since we were also running out of PCR primer mix, Vincent went ahead and made some more.  
In order to continue with the production of T7 promoter variants, Vincent had to make more gene-specific Lysis (i.e. T4 Lysis with RBS upstream). For this, Vincent used the new Hifi+ enzyme that had been ordered the previous day. Since we were also running out of PCR primer mix, Vincent went ahead and made some more.  
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== Friday, 26 August ==
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== Friday, 26 August 2011 ==
Vincent ran a plate-reader experiment for the K1-T7-lysis BL21 cells. The first three rows received various doses of IPTG before the experiment got under way. The next three rows (const, lac, lac2) received no IPTG for the first 2 hours of incubation but then were given the same IPTG doses as the first three rows. Data analysis will take place tomorrow.  
Vincent ran a plate-reader experiment for the K1-T7-lysis BL21 cells. The first three rows received various doses of IPTG before the experiment got under way. The next three rows (const, lac, lac2) received no IPTG for the first 2 hours of incubation but then were given the same IPTG doses as the first three rows. Data analysis will take place tomorrow.  
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Vincent made a Gibson assembly of the 18 T7-RFP promoter variants and the 3 T7-Lysis variants into the K1 backbone. The DNA will be transformed on Saturday.  
Vincent made a Gibson assembly of the 18 T7-RFP promoter variants and the 3 T7-Lysis variants into the K1 backbone. The DNA will be transformed on Saturday.  
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Nadine made colony PCRs for yesterday's Gibson assemblies: J61002 Plac-RFP and pSB3K1 TetR-LacI; she also made PCRs for pSB3K1 TetR-LacI that had been sent for sequencing on wednesday. Unfortunately, the plate with J61002 Plac-lysis yielded no colonies...
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Details of the PCRs:
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* pSB3K1 TetR-LacI:
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** amplify LacI with sequencing primers
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** amplify TetR with sequencing primers
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* J61002 Plac-RFP:
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** amplify RFP with colony PCR primers
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** amplify RFP with Gibson primers
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With the sequencing primers, one of them binding in the middle of RFP, all 6 colony tested gave positive results. Strangely, there seems to be 2 bands with a slight difference in size. With the Gibson primers that contain Plac, colonies 1 and 3 have a brighter band. Either they are the only positive ones, or they just have a bigger amount of DNA (as also seen on the other gel).
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For pSB3K1, both PCRs failed. Since it's very unlikely that we have a plasmid that lost TetR, there must have been a problem in the PCR; it will be repeated.
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Nadine also digested the (supposed) J61002 Plac-RFP plasmids from Tuesday's Gibson assembly: colony 6 from Gibson plate that was red, colony 9 from Gibson plate that was white and colony 12 from negative control plate that was also red. Pst1 has a restriction site in the original J61002 backbone, therefore it should cut independently of RFP insertion. The results indicate that only colony 9 was digested by the enzyme, therefore it's likely that the red colonies contain an unknown plasmid...
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Revision as of 09:22, 27 August 2011