Team:EPF-Lausanne/Notebook/July2011

From 2011.igem.org

(Difference between revisions)
(Tuesday, 12 July 2011)
(Monday, 11th of July 2011)
Line 141: Line 141:
* T4 lysis cassette on registry plasmid, final concentration: 29.7 ng/ul
* T4 lysis cassette on registry plasmid, final concentration: 29.7 ng/ul
* RFP amplification with Plac from Gibson J61002 plasmid, final concentration: 61,2 ng/ul
* RFP amplification with Plac from Gibson J61002 plasmid, final concentration: 61,2 ng/ul
-
 
-
 
-
Then we made 2 Gibson assemblies, transformed cells and plated them on ampicillin dishes. The newly assembled vectors will have ampicillin resistance, LacI under Ptet plus either lysis under Plac or RFP under Plac.
 
Line 153: Line 150:
[[File:EPFL_20110711_J61002-Ptet-digestion.jpg|600 px]]
[[File:EPFL_20110711_J61002-Ptet-digestion.jpg|600 px]]
-
 
== Tuesday, 12 July 2011 ==
== Tuesday, 12 July 2011 ==

Revision as of 19:35, 12 July 2011