Team:Paris/August 20
From 2008.igem.org
(Difference between revisions)
(→Screening) |
(→Sequencing) |
||
Line 489: | Line 489: | ||
*We succeed for FlgA promoter | *We succeed for FlgA promoter | ||
*FlgB and flhB don't match with our expected sequences. We decided to cut our Miniprep product with other enzymes to check our sequence. | *FlgB and flhB don't match with our expected sequences. We decided to cut our Miniprep product with other enzymes to check our sequence. | ||
- | |||
=='''Digestion'''== | =='''Digestion'''== |
Revision as of 17:44, 5 September 2008
Screening of the cloning of E0240 and FlhDC+promotorSpreading the clones in order to obtain single colonies
The plates obtained from the speading of yesterday can't be used because there are not single colonies.
Miniprep and stock glycerolConstruction for FIFOAim : Construction of pFlgA - YFP tripart (+/- LVA) "pFlgA-RBS-YFP-dbl ter" (pFlgA-E0430/E0432) DigestionMeasurement of concentration of minipreps
Digestion
Gel Extraction
=> Following a mistake, the right E0430(D166) and E0432(D167) digestion, have not been purified. Construction of: promotor-rbs-LasR-dbl terResults of the transformation we did the day before yesterdayNumber of colonies
PCR Screening
Minipreps
Promoter characterization plasmidsLigationOur ligations from yesterday didn't work. The positive control for transformation worked. DigestionWe had a problem with a gel extraction so we have to make again the digestions from yesterday, Other digestions made:
Sequencing
*We succeed for FlgA promoter *FlgB and flhB don't match with our expected sequences. We decided to cut our Miniprep product with other enzymes to check our sequence. Digestion
ScreeningGel 1
Gel 2
Conclusion => the sequence of pFlgB and pFlhB are not good we will tried to isolate pFlhB again. |