Team:EPF-Lausanne/Notebook/August2011

From 2011.igem.org

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(Friday, 26 August 2011)
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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 that has RFP... Since colony 9 was positive for RFP colony PCR, it can be our expected plasmid that has little expression 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 plasmid that has little expression of RFP.
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== Saturday, 27 August 2011 ==
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Nadine did a second colony PCR on the pSB3K1 TetR-LacI colonies. This time, the LacI PCR worked for all samples (fragment should be about 750 bps), but the TetR PCR failed again (although these primers already worked in the past). One colony will be sent for sequencing on Monday.
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Revision as of 16:49, 27 August 2011