Team:INSA-Lyon/Project/Stage3/Strategy

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Revision as of 15:05, 27 October 2010 by Magalbrun (Talk | contribs)





Strategy


We chose to follow two differents strategies to obtain our systems of regulation.



Thermoregulation


For this system of regulation, we decided to synthesized directly the sequence of the curli promoter with the igem restriction sites. In the same time a part with the gene ompR234 is created by PCR, from the genome of the chassi PHL818. Then we ligate an igem reporter gene with the curli promoter and we wanted to make a double transformation with ompR234 to see if our parts work as we hoped.


curli 14K ou curli 22B construction finale


Curli and reporter gene ligation



Constitutive gene and OmpR234 ligation construction finale


Constitutive gene and OmpR234 ligation



The final plasmid construction of the thermometer RNA will contain a constitutive promoter(BBa_J23119), the thermometer RNA, the PPI-protein fused and a terminator.



Control under Arabinose



In this part we decided to realize three different constructions to control the regulation. The first one consists in the constitutive production of LuxR and LuxI proteins to control the promoter LuxR/HSL. The second one is the construction with the promoter LuxR/HSL to control the expression of the operon PhaCAB To finish a construction with Pbad/araC, which is a promoter whose activity depends on addition of arabinose in medium. In this case, the promoter influences the synthesis of a cI repressor and a phasin-intein construction. The cI repressor is isolated from bacteriophage λ and negatively regulates the activity of the LuxR/HSL regulated promoter.


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