Team:EPF-Lausanne/Notebook/July2011

From 2011.igem.org

(Difference between revisions)
(Monday, 25 July 2011)
(Monday, 25 July 2011)
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[[File:EPFL-2011-07-25_Gibson_TD_PCR_HifiPLUS.jpg|thumb|right|Gibson fragments for the reporter plasmid, PCR'd with HifiPLUS enzyme. Good yield, but unexpected product sizes.]]
[[File:EPFL-2011-07-25_Gibson_TD_PCR_HifiPLUS.jpg|thumb|right|Gibson fragments for the reporter plasmid, PCR'd with HifiPLUS enzyme. Good yield, but unexpected product sizes.]]
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Alessandro ran the Gel on Friday's PCR - that made Gibson fragments for the reporter plasmid, using the HifiPLUS enzyme. There is definitely some product (whereas iProof yields nothing at all), but the bands are of unexpected sizes. Only LacI seems to have worked properly. There was probably a mixup or some similar problem with the other PCRs. In conclusion: our '''iProof enzyme seems not to work ''', either because it degraded, or it is just not suitable for this type of experiment. We should now use another enzyme. We ordered some Hifi+ for the next PCRs.
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Alessandro ran the Gel on Friday's PCR - that made Gibson fragments for the reporter plasmid, using the HifiPLUS enzyme. There is definitely some product (whereas iProof yields nothing at all). LacI and RFP seem to have worked properly. The lysis fragment is possibly a little short, and the backbone band is way too small. Overall, except for the backbone, it worked well. Douglas will try a gradient PCR for the backbone and Lysis device. It might help debug the backbone PCR. We aren't too worried about the short lysis fragment - that gel is overall wierd, so that could be the problem.
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In conclusion: our '''iProof enzyme seems not to work ''', either because it degraded, or it is just not suitable for this type of experiment. We should now use another enzyme. We ordered some Hifi+ for the next PCRs.
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Revision as of 15:39, 25 July 2011