Team:Grenoble-EMSE-LSU/Project/Modelling

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<p>Modelling took a large place in the project. We used modelling for the characterization of KillerRed and the Voigt plasmids and also needed it for the control of the a bacterial population. With our device, we cannot control a population of living cells with a simple closed-loop transfer function. The first reason is that optical measurements (OD at 600 nm or fluorescence) originate from all cells, whether they are alive or not. As a consequence, it is not easy to reconstruct the size of a population of living cells from a fluorescent intensity or an $OD_{600}$ reading. Second, there is a large delay between an action and its effect: there are about one or two hours between the onset of illumination and a decrease in fluorescence intensity augmentation speed. In those conditions, a simple closed-loop transfer function is predictably unstable, and a predictive model control is needed to stabilize the population of living cells.</p>
<p>Modelling took a large place in the project. We used modelling for the characterization of KillerRed and the Voigt plasmids and also needed it for the control of the a bacterial population. With our device, we cannot control a population of living cells with a simple closed-loop transfer function. The first reason is that optical measurements (OD at 600 nm or fluorescence) originate from all cells, whether they are alive or not. As a consequence, it is not easy to reconstruct the size of a population of living cells from a fluorescent intensity or an $OD_{600}$ reading. Second, there is a large delay between an action and its effect: there are about one or two hours between the onset of illumination and a decrease in fluorescence intensity augmentation speed. In those conditions, a simple closed-loop transfer function is predictably unstable, and a predictive model control is needed to stabilize the population of living cells.</p>
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Revision as of 11:13, 4 October 2013

Grenoble-EMSE-LSU, iGEM


Grenoble-EMSE-LSU, iGEM

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