Team:Paris/August 16
From 2008.igem.org
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*10 µL of template DNA in 50 µL of pure water | *10 µL of template DNA in 50 µL of pure water | ||
*Blank : 10 µL of EB buffer in 50 µL of water. | *Blank : 10 µL of EB buffer in 50 µL of water. | ||
- | {| | + | {||- style="text-align: center;" border="1" |
|align="center"|'''Digestion name''' | |align="center"|'''Digestion name''' | ||
|align="center"|'''What's in ?''' | |align="center"|'''What's in ?''' | ||
|'''Enzymes''' | |'''Enzymes''' | ||
- | |align="center"|'''DNA | + | |align="center"|'''DNA C° (ng/µL)''' |
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|align="center"|D 158 | |align="center"|D 158 |
Revision as of 17:49, 3 September 2008
Construction of OmpR*+RBS and EnvZ*+RBS: LigationsCleaning of the DNA after the digestionWe used the QIAcube to wash the DNA, following the standard protocol. Measure of DNA concentration of the digestion productsWe used the biophotometer.
List of ligations
Creation of a registry of pFliL, pFlhDC, and FlhDCAnalysis of the transformation we did yesterdayL143, L144, T1 and T2 showed no colonies. The positive control with pUC19 worked well.
Cleaning of the DNA after the digestionWe used the QIAcube to wash the DNA, following the standard protocol. Measure of DNA concentration of the digestion productsWe used the biophotometer.
List of ligations
Construction of pLas-TetR-GFP tripart & rbs-LasR-dble terTransformation
Digestion check from yesterday
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