Team:EPF Lausanne/Next steps

From 2013.igem.org

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{{Template:EPFL2013Header}}
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Up until now we succeded  
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Up until now we succeded<br\>
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• Producing Nanoparticles and loading them
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• Producing Nanoparticles and loading them<br>
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• Clone a pH sensitive promoter
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• Clone a pH sensitive promoter<br>
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• Engineer a fusion protein between ice nucleation protein and Streptavidin
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• Engineer a fusion protein between ice nucleation protein and <br>
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<br\>
But we weren’t able to characterize and assemble the parts completely.
But we weren’t able to characterize and assemble the parts completely.
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<br\>
==What we would have done with more time:==
==What we would have done with more time:==
==Nanoparticles==
==Nanoparticles==
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<br>
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<br>
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<br>
==Cell surface display of Streptavidin==
==Cell surface display of Streptavidin==
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• Cloned a plasmid that encodes a fusion protein INP-Streptavidin-YFP and one INP-YFP-Streptavidin. Then we would have been able to use the exact same protocol we used to characterize the Biobrick BBa_K523013, to proof surface localization.
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• Cloned a plasmid that encodes a fusion protein INP-Streptavidin-YFP and one INP-YFP-Streptavidin. Then we would have been able to use the exact same protocol we used to characterize the Biobrick BBa_K523013, to proof surface localization.<br>
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•  
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<br>
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<br>
==Sensing/Effector==
==Sensing/Effector==
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<br>
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<br>
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<br>
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==Device==
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==Taxi.Coli==
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• Cloned one of our Biobricks in a backbone that contains another resistance than chloramphenicol to cotransfect bacteria with the Plasmids responsible for Sensing/Effector and the Plasmid used to connect the Nanoparticles.
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• Cloned one of our Biobricks in a backbone that contains another resistance than chloramphenicol to cotransfect bacteria with the Plasmids responsible for Sensing/Effector and the Plasmid used to connect the Nanoparticles.<br>
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•  
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<br>
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<br>
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Revision as of 08:45, 4 October 2013

Taxi.Coli: Smart Drug Delivery iGEM EPFL

Header

Up until now we succeded
• Producing Nanoparticles and loading them
• Clone a pH sensitive promoter
• Engineer a fusion protein between ice nucleation protein and

But we weren’t able to characterize and assemble the parts completely.

Contents

What we would have done with more time:

Nanoparticles




Cell surface display of Streptavidin

• Cloned a plasmid that encodes a fusion protein INP-Streptavidin-YFP and one INP-YFP-Streptavidin. Then we would have been able to use the exact same protocol we used to characterize the Biobrick BBa_K523013, to proof surface localization.


Sensing/Effector




Taxi.Coli

• Cloned one of our Biobricks in a backbone that contains another resistance than chloramphenicol to cotransfect bacteria with the Plasmids responsible for Sensing/Effector and the Plasmid used to connect the Nanoparticles.



Wiki Links

Retrieved from "http://2013.igem.org/Team:EPF_Lausanne/Next_steps"