ULB/13 August 2009



 iGEM Team:ULB-Brussels Wiki  

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Université Libre de Bruxelles

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 Home Team Project</a></li> Parts</a></li> Safety</a></li> Notebook</a></li> Sponsors</a></li> </ul> <ul>

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{| align="right"

Manipulation on plasmides

 * Bacteria with the plasmid with RBS (BBa_B0034) growed.
 * The ligation of the promoter-RBS-plasmid (chloramphenicol resistant) didn't work: the reason could be the use of the protocol of manual assembly, who told us to leave league 10 minutes at room temperature, then deactivate the enzymes, insted of 24 hours by the T4 ligase guide.
 * Verify that the bricks are now in the medium of our extractions: Digestion of the promoter and promoter + RBS by restriction enzymes EcoRI and Spel, RBS + RFP and the terminator by XbaI and PstI.
 * We made a PCR with primers for ccdA program received at 55 ° C then a gel migration.

Results



 * Verification of bricks:4 DNA primers "normal", white primers "normal", 4 DNA primers reverse, white reverse primers.


 * PCR: all tubes have succeeded except the one control sample which is out of place (4th position instead of 6th).