Team:EPF-Lausanne/Notebook/August2011

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(Difference between revisions)
(Friday, 26 August 2011)
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[[File:EPFL_Igem_2608_j6RFPcol24.jpg|thumb|300px]]
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[[File:EPFL_Igem_2608_pcr13.jpg|thumb|300px]]
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...
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...
Details of the PCRs:
Details of the PCRs:
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** amplify RFP with colony PCR primers
** amplify RFP with colony PCR primers
** amplify RFP with Gibson primers
** 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).
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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[[File:EPFL_Igem_2608_J6RFP_dig.jpg|thumb|300px]]
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 that has RFP... Since colony 9 was positive for RFP colony PCR, it can be our expected plasimid that has little transcription of RFP.
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 that has RFP... Since colony 9 was positive for RFP colony PCR, it can be our expected plasimid that has little transcription of RFP.
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Revision as of 09:29, 27 August 2011