Team:EPF-Lausanne/Our Project/Summary

From 2011.igem.org

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(Characterisation)
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[[File:EPFL-MITOMI shot.png|400px]]
[[File:EPFL-MITOMI shot.png|400px]]
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''' 3) determining the binding of each mutant to the wild-type TetO sequence ''in vivo''
''' 3) determining the binding of each mutant to the wild-type TetO sequence ''in vivo''
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[[File:EPFL_Nadine-exp3-induction.png|600px]]
[[File:EPFL_Nadine-exp3-induction.png|600px]]
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''' 4) comparing the results of both characterization
''' 4) comparing the results of both characterization
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We were able to change the specificity of some of our mutants; however this change was not big enough to have a fully orthogonal mutant that would not recognize the wild-type consensus sequence.
We were able to change the specificity of some of our mutants; however this change was not big enough to have a fully orthogonal mutant that would not recognize the wild-type consensus sequence.
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== DIY Microfluidics ==
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In parallel to the work on the transcription factor pipeline, we built a computer-controlled microfluidic injection setup from off-the shelf components, to demonstrate that microfluidics can be used for less than $1000. To help future teams from other universities get started with microfluidics, we wrote on our wiki instructions to replicate the setup.
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In addition to this, we programmed a web interface for the machine: from any web browser, users can view a live video feed from the microscope that images the chip, and control the valves by clicking buttons on the web page. Concurrent use is managed by a queue system. The web site was mostly used at the Jamboree in Amsterdam to illustrate the principle of microfluidics to other iGEMers, then it stayed live for most of October, allowing anybody to try the setup. The demonstration chip had channels in the shape of the iGEM logo, and was filled with a red and a blue dye to highlight flow and mixing.
{{:Team:EPF-Lausanne/Templates/Footer}}
{{:Team:EPF-Lausanne/Templates/Footer}}

Revision as of 22:18, 28 October 2011