Team:Tokyo Tech
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- | <div><b><font size=4>We want to make a <i style='mso-bidi-font-style:normal'> | + | <div><b><font size=4>We want to make a <i style='mso-bidi-font-style:normal'>coli Touch!!</i></font></b></div> |
<p>To make a Coli Touch, we use input style of pressure.</p></td> | <p>To make a Coli Touch, we use input style of pressure.</p></td> | ||
<td> | <td> |
Revision as of 16:25, 26 October 2008
Basic project | Aplication project |
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Parts Submitted to the Registry | Our Team | Acknowledgements |
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Basic project
We want to make a coli Touch!!
To make a Coli Touch, we use input style of pressure. |
Why pressure?
First, there were various ways as input.
For example, small molecule, heat, and light were used until iGEM 2007.
But no one used pressure as input.
Moreover, past way(small molecule, heat and light) are difficult to induct uniformly.
Pressurize can induct unifomly.It's prospect of technological application in confirmatory experiment. |
We use pressure sensitive parts.
One paper says "One promoter is sensitive to pressure.". So we focused on it. |
Confirmatory experiment
Construction
For confirming pressure-response ability of pressure-inducible promoter, we experimented under 0.1MPa and 30MPa pressure. We chose TetR promoter(PtetR) as pressure-inducible promoter and we constructed two plasmids - one is PtetR-GFP on pSB6([http://partsregistry.org/Part:BBa_K121010 BBa_K121010]), the other is promoter less-GFP on pSB6([http://partsregistry.org/Part:BBa_K121013 BBa_K121013]) as a negative control.
Experiment under high pressure
Dilute this culture medium by 1% by adding fresh medium and suitable antibiotic (ampicilin; 50㎍/ml). Next, seal this culture medium with oxygen-saturated fluorinert (25% volume of medium) in polypropylene tubes with parafilm (figure3). Put this tube into pressure vessel filled with water (figure4). Next cup pressure vessel. Finally, pressurize pressure vessel by pressure device(figure5). and then incubation was started at 37℃ immediately at each pressure vessel(original designed) for 16h at 37℃.After cultivation(figure6), the cells were examined by fluorescence microscope.
Result
The result was that PtetR activity under 30MPa pressure is about 2.5 times stronger than PtetR activity under 0.1MPa pressure. Therefore, we confirmed that PtetR was induced under 30MPa pressure.
Acrylic container
We create devices for confirming pressure response of lac promoter. This is the first step of creating touch display. This device made of Acrylic glasses and has two holes (show figure). Each hole contains tubes and water. Inside tubes E. coli is cultivated. Pressure can travel to inside tubes. One hole (A) is covered with a plastic tape (show figure). Therefore the hole is pressurized.The other (B) is covered with a block made of an acrylic glass. (show figure) Therefore the hole is not pressurized by water. |
E.coli type in tubes |
* “Ptet” on pSB6 plasmid (E.coli strain; JM109) |
After pressurized the container, we observed the E.coli by a fluorescence microscope. The result shows below. |