Team:LCG-UNAM-Mexico/Wet Lab/Experiments
From 2009.igem.org
(Difference between revisions)
(→asRNA) |
(→Multipromoter) |
||
Line 56: | Line 56: | ||
This result was only for T7 RNA polymerase but we are planning to implement a better assay system to include a WT T3 & T7 | This result was only for T7 RNA polymerase but we are planning to implement a better assay system to include a WT T3 & T7 | ||
- | RNA polymerase, a plasmid that have GFP and not the multipromoter and a strain that | + | RNA polymerase, a plasmid that have GFP and not the multipromoter and a strain that have our multipromoter and not T7 RNA polymerase. Also we need to clone the biocrick in a plasmid that only contain our multipromoter and no other in the same direction in order to avoid licking from near upstream promoters, this is important because we are using quite toxic bacterial proteins that will be induced under the presence of T3 or T7 so estimation of the basal transcription its important to test the viability of our death system. |
- | we need to clone the biocrick in a plasmid that only | + | |
- | that will be induced under the presence of T3 or T7 so | + | |
- | the viability of our death system. | + | |
====Quorum sensing system==== | ====Quorum sensing system==== |
Revision as of 23:52, 21 October 2009