Team:LCG-UNAM-Mexico/Experiments/Design
From 2008.igem.org
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<strong>15.-Y. Dong and L. Zhang, “Quorum sensing and quorum-quenching enzymes”.2005.</strong> | <strong>15.-Y. Dong and L. Zhang, “Quorum sensing and quorum-quenching enzymes”.2005.</strong> | ||
- | + | <p align="left"><strong>16.-N.T. Keen, S. Tamaki, D. Kobayashi, and D. Trollinger. 1998. </strong> | |
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Revision as of 06:32, 29 October 2008
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System First of all, we needed a system that could cause a change in its medium conductivity. An extrusion pump seemed to be the best way to achieve this. Once this was devised, we needed a way to regulate the system. We decided to use a negative regulator because it's the only way to transcriptionally regulate the expression of a gene in a definitive way.
The components selected to fulfill the system requirements are enlisted in the next table:
Devices
Device BBa_K119009: The extrusion pump.
Devices BBa_K119010/BBa_K119011: The regulatory device In order to control the RcnA activity this device includes the gene encoding LuxR under the regulation TetR constitutive promoter followed by cI, which will repress RcnA in the prescence of AHL:LuxR. The last component of the device is the gene encoding AiiA. In BBa_K119010 lacZ promoter is upstream of AiiA, while BBa_K119011 carries a mutated version of it. The plasmid carrying this device will be PRK415.
References
2.-Rodrigue A. Et al.”Identification of rcnA (yohM), a Nickel and Cobalt Resistance Gene in Esherichia coli” 2005. 3.-Kovach et al.,”pBBR1MCS: a broad-host-range cloning vector”.1994 4.- 5.-link a chiba, ahorita lo pongo 6.-Whiteheada N.A., Barnada A.M.L., Slaterra H..”Quorum-sensing in Gram-negative bacteria”2001. 16.-N.T. Keen, S. Tamaki, D. Kobayashi, and D. Trollinger. 1998.
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