Team:Goettingen/Focus Groups

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In this group it´s all about creating a selection system that enables selecting the <i>E. coli</i> clones that are able to swim the fastest. In an extensive literature search we have collected different swimming media and swimming assays and have evaluated them with regard to our goal. The media can differ in various ways from each other and in our case the most important ones are the agar concentration and the nutrient content. The agar concentration has to be low enough to make swimming possible but high enough to form a semisolid structure. The nutrient content hast to be as low as possible without significantly inhibiting growth because the <i>E. coli</i> cells will only start to swim when there are no more nutrients in their current place. The low nutrient content is also necessary to observe whether a directed taxis in dependence on our tested molecule occurs. Through all these different experiments we will be able to set up a selection system that is quick, easy to handle and delivers reproducible results.  
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In this group it is all about creating a selection system that enables selecting the <i>E. coli</i> clones that are able to swim the fastest. In an extensive literature search we have collected different swimming media and swimming assays and have evaluated them with regard to our goal. The media can differ in various ways from each other and in our case the most important ones are the agar concentration and the nutrient content. The agar concentration has to be low enough to make swimming possible but high enough to form a semisolid structure. The nutrient content hast to be as low as possible without significantly inhibiting growth because the <i>E. coli</i> cells will only start to swim when there are no more nutrients in their current place. The low nutrient content is also necessary to observe whether a directed taxis in dependence on our tested molecule occurs. Through all these different experiments we will be able to set up a selection system that is quick, easy to handle and delivers reproducible results.  
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In this group, the main focus is to first clone the aspartate receptor TAR from <i>E. coli</i> under different strong constitutive promoters
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In this group, the main focus is to first clone the aspartate receptor Tar from <i>E. coli</i> under different strong constitutive promoters
into vectors. After examination of effects overexpressing this chemotaxis receptor, the next challenge is to mutagenize this protein to receive
into vectors. After examination of effects overexpressing this chemotaxis receptor, the next challenge is to mutagenize this protein to receive
a chemoreceptor library. Ideally, the specificity of the receptor becomes altered due to mutation of the ligand binding sites important for chemical binding.
a chemoreceptor library. Ideally, the specificity of the receptor becomes altered due to mutation of the ligand binding sites important for chemical binding.

Revision as of 16:10, 17 September 2012