Team:UC Chile2/Cyanolux/Project

From 2012.igem.org

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<h1>Goal</h1>
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<h1>Main Goal</h1>
<p>Natural cycles have always fascinated mankind, probably due to the mysterious mechanisms involved in them and the power they exert in our everyday life. Since the dawn of synthetic biology, engineering oscillatory systems has been a recurrent topic, being Ellowitz's represillator a classical example. Nevertheless, to date no iGEM team has accomplished the implementation of a robust oscillatory system. That will be our challenge for this year's iGEM project.</p>
<p>Natural cycles have always fascinated mankind, probably due to the mysterious mechanisms involved in them and the power they exert in our everyday life. Since the dawn of synthetic biology, engineering oscillatory systems has been a recurrent topic, being Ellowitz's represillator a classical example. Nevertheless, to date no iGEM team has accomplished the implementation of a robust oscillatory system. That will be our challenge for this year's iGEM project.</p>
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<p>This constructs is an integrative plasmid which targets neutral recombination sites (slr0370 and sll0337). We selected this locus because it has been extensively used in the literature (REFERENCE) and it shown to have no deleterious effects on Synechocystis viability. We selected Kanamycin resistance as our transformation marker. [PUT LINK TO CONSTRUCT HERE].</p>
<p>This constructs is an integrative plasmid which targets neutral recombination sites (slr0370 and sll0337). We selected this locus because it has been extensively used in the literature (REFERENCE) and it shown to have no deleterious effects on Synechocystis viability. We selected Kanamycin resistance as our transformation marker. [PUT LINK TO CONSTRUCT HERE].</p>
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<h4>LuxAB under the transaldolase promoter</h4>
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We have choose the transaldolase promoter to express the luciferase part of the operon, as in the literature the promoter is described as having a peak of expression at 2 hours past dusk, which we believe is just the right timing to "turn on the lamp".
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We've found 2 versions of the Bacterial luciferase which we intend to use on this construct. The first one is from Photorhabdus luminiscence K216008 from the 2009 Edinburgh iGEM team and the second one is part from the LuxBrick (K325909 from the 2010 Cambridge iGEM team) and originally comes from Vibrio fisherii but has been "E.coli optimized".
<h3>pSB1C3_IntS</h3>
<h3>pSB1C3_IntS</h3>
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<p>Alternatively, we designed our LuxCDEG contructs for the Utah 2010 iGEM Team plasmid backbone . [http://partsregistry.org/wiki/index.php?title=Part:BBa_K390200 pSB1A2_IntC].</p>
<p>Alternatively, we designed our LuxCDEG contructs for the Utah 2010 iGEM Team plasmid backbone . [http://partsregistry.org/wiki/index.php?title=Part:BBa_K390200 pSB1A2_IntC].</p>
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<h1>References</h1>
<h1>References</h1>

Revision as of 02:40, 24 September 2012

Project: Luxilla - Pontificia Universidad Católica de Chile, iGEM 2012