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<div class="text"> Kinetics Model </div> | <div class="text"> Kinetics Model </div> | ||
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<p>The last modeled portion of the project used the Flux Balance Analysis tool to predict the growth rate of the E. coli cells on the sole carbon source of PET. The original matrix and parameters where downloaded from the CoBRA toolbox iJO1366 model [ ]. The model was then expanded to include this new pathway and genes and then the system was optimized for biomass growth and the objective value was proportional to the growth rate of the bacteria. | <p>The last modeled portion of the project used the Flux Balance Analysis tool to predict the growth rate of the E. coli cells on the sole carbon source of PET. The original matrix and parameters where downloaded from the CoBRA toolbox iJO1366 model [ ]. The model was then expanded to include this new pathway and genes and then the system was optimized for biomass growth and the objective value was proportional to the growth rate of the bacteria. | ||
FBA uses a stochastic matrix of the all the metabolisms’ chemical reactions and optimizes these various equations to produce a unit of biomass, which is inferred as another metabolite of the system. The general form of the model is:<br/ > | FBA uses a stochastic matrix of the all the metabolisms’ chemical reactions and optimizes these various equations to produce a unit of biomass, which is inferred as another metabolite of the system. The general form of the model is:<br/ > | ||
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<div class="text"> Metabolism Model </div> | <div class="text"> Metabolism Model </div> | ||
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<h3>Genetics Model </h3> | <h3>Genetics Model </h3> | ||
<p>The genetics system used in our experiments has the degradation of PET and the assimilation of PET carbons in the cell on two separate plasmids. The relevant amounts of copies of the 6 enzyme genes and their rates of change were described in differential equations. The different promoter interactions of each plasmid were also taken into account and the secretion of mechanisms for PETase and/or MHETase were also included, to help us predict the amount of enzymes breaking down the PET. Click on the plasmid and genetics section to read about our description. </p> | <p>The genetics system used in our experiments has the degradation of PET and the assimilation of PET carbons in the cell on two separate plasmids. The relevant amounts of copies of the 6 enzyme genes and their rates of change were described in differential equations. The different promoter interactions of each plasmid were also taken into account and the secretion of mechanisms for PETase and/or MHETase were also included, to help us predict the amount of enzymes breaking down the PET. Click on the plasmid and genetics section to read about our description. </p> | ||
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<p>Example of the Genetics Model</p> | <p>Example of the Genetics Model</p> | ||
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<img src="https://static.igem.org/mediawiki/2018/c/ce/T--RHIT--GeneticExampleonPicture.png" style="width:450px;height:275px;"> | <img src="https://static.igem.org/mediawiki/2018/c/ce/T--RHIT--GeneticExampleonPicture.png" style="width:450px;height:275px;"> | ||
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<img src="https://static.igem.org/mediawiki/2018/2/28/T--RHIT--GeneticsExEqs.png" style="width:500px;height:180px;"> | <img src="https://static.igem.org/mediawiki/2018/2/28/T--RHIT--GeneticsExEqs.png" style="width:500px;height:180px;"> | ||
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<div class="text"> Genetics Model </div> | <div class="text"> Genetics Model </div> | ||
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Revision as of 16:10, 9 July 2018