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+ | <h2>OUR DESIGN</h2> | ||
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+ | We have chosen protein from the luxI and luxR protein family to build our parts, which is the most common family of acyl homoserine lactone (AHL) autoinducer-receptor system. The luxI gene encodes for an autoinducer synthase that catalyses the formation of the acyl homoserine lactone from the acyl-S-adenosylmethionine intermediate, [1] which is then secreted and binded to transcription factors encoded by the luxR gene. Being activated, a luxR complex can bind the promotor with a DNA binding region near its N-terminal and initiate the ranscription process of downstream CDA genes. | ||
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+ | In our construction (see fig.2), the system is regulated by both lac operon and AHL signalling pathway. Our PluxlacO promoter can both respond to lacI repressors and luxI regulator. Under the presence of IPTG, which is the key to both the quorum sensing system and expression of our CDA protein, repression is removed and transcription of both luxI and luxR is initiated. The two plasmid vectors, pTA1109 and pTA1083, serve as a translation regulator carrier and target gene carrier, respectively. </p> | ||
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+ | Under low cell density, transcription of the CDA gene on pTA1083 is repressed by inactivate promotor and all unwanted background expression is repressed. After the threshold concentration is passed, the presence of AHL promotes both the transcription of CDA genes as well as the luxI gene—which in turn produces more AHL in intracellular space and creates a positive feedback loop that eventually raises the transcription level of CDA genes rapidly and dramatically.</p> | ||
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Revision as of 12:07, 17 October 2018