Team:Oxford/Results
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- | + | <p> Wetlab Results: <br><br> | |
- | For the | + | For the bioremediation aspect of DCMation, we have managed to:<br><br> |
1. purify the pUNI-ABTUNJK and pSB1C3-ABTUNJK plasmids, which encode the microcompartments<br> | 1. purify the pUNI-ABTUNJK and pSB1C3-ABTUNJK plasmids, which encode the microcompartments<br> | ||
2. verify expression of pUNI-ABTUNJK plasmids in E. coli using Western blotting<br> | 2. verify expression of pUNI-ABTUNJK plasmids in E. coli using Western blotting<br> | ||
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8. insert the microcompartment-tagged sfGFP into pME6010, and used fluorescence microscopy to image this<br> | 8. insert the microcompartment-tagged sfGFP into pME6010, and used fluorescence microscopy to image this<br> | ||
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+ | Realisation Results: <br><br> | ||
+ | For the containment of our bacteria, we have managed to: <br><br> | ||
+ | 1. synthesise novel agarose beads that have a polymeric coating which limits DCM diffusion into the beads. This allows optimum degradation by the bioremediation bacteria, while physically containing the bacteria for safety reasons <br> | ||
+ | 2. use computer-aided modelling to design a prototype of the DCMation system, and physically constructed this container <br> | ||
+ | 4. 3D print a cartridge to hold our biosensor bacteria, which can easily be replaced by the user<br> | ||
+ | 5. construct a prototype circuit that lights up when the photodiodes detect light emission from our biosensing bacteria that are contained in the cartridge. This lets the user have a simple yes/no response to whether the contents of the container are safe for disposal.<br> | ||
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Revision as of 15:23, 16 October 2014