Team:EPF-Lausanne/Notebook/July2011

From 2011.igem.org

(Difference between revisions)
(Wednesday, 13 July 2011)
(Wednesday, 13 July 2011)
Line 180: Line 180:
[[File:EPFL-2011-07-13_Stitch_PCR.jpg|thumb|First result from the fusion PCR: tetR mutant EA37 appears in "detectable" amounts]]
[[File:EPFL-2011-07-13_Stitch_PCR.jpg|thumb|First result from the fusion PCR: tetR mutant EA37 appears in "detectable" amounts]]
-
Douglas purified the gels containing yesterday's mutation-PCR products, following the XXX protocol XXX. Isopropanol was added to the "Common PCR" product, as its expected length is inferior to 500bp. The final DNA concentrations, measured by photospectrometry, are listed in the following table:
+
Douglas purified the gels containing yesterday's mutation-PCR products, following the XXX protocol XXX. Isopropanol was added to the "Common PCR" product, as its expected length is inferior to 500bp. The final DNA concentrations, measured by photospectrometry, are listed in the following table. Even the very low concentration of YF36 should be sufficient for a PCR template, and the weird "260/280" ratio apparently results from agarose gel residues.
{|
{|

Revision as of 16:12, 13 July 2011