Team:Austin Texas/kit
From 2014.igem.org
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[[File:Alex and Foil-covered incubator.jpg|200px|thumb|right|Protection of light-sensitive ncAAs using a foil-wrapped incubator.]] | [[File:Alex and Foil-covered incubator.jpg|200px|thumb|right|Protection of light-sensitive ncAAs using a foil-wrapped incubator.]] | ||
- | An ncAA synthetase/tRNA pair was cloned into pStG and transformed into pFRYC amberless ''E. coli'' | + | An ncAA synthetase/tRNA pair was cloned into pStG and transformed into pFRYC amberless ''E. coli'' and pFRY amberless ''E. coli''. Other necessary control strains include RFP amberless ''E. coli'' (RFP control), sfGFP amberless ''E. coli'' (GFP control), amberless ''E. coli'' (cell background control), and LB media supplemented with ncAA (media background control). An overnight culture of each strain was grown in LB with the appropriate antibiotics at 37ºC and 225rpm. 10 mL of media with the appropriate antibiotics was inoculated with 100 µL of overnight culture and allowed to grow in the same conditions until the culture density was ~0.2-0.3 OD, or ~3 hours. The 10 mL culture was split between 4 different sterile test-tubes, 2 mL of culture per tube. The conditions of the four test tubes were as follows: |
*-IPTG,-ncAA | *-IPTG,-ncAA | ||
*-IPTG,+ncAA | *-IPTG,+ncAA | ||
*+IPTG, -ncAA | *+IPTG, -ncAA | ||
*+IPTG, +ncAA | *+IPTG, +ncAA | ||
- | IPTG | + | If the cultures did not have IPTG or an nCAA, an equal volume of sterile deionized water was added in order to keep the volumes between cultures constant. Once the water, the IPTG, and the ncAA were added appropriately, the cultures were allowed to grow to ~0.5 OD 600. 70 µL of each culture condition and control culture were added to a separate well in a transparent 96-well plate for fluorescence and OD readings using a fluorometer. |
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[[File:10-14-14 big experiment test tubes.png|450px|thumb|left| Preparation for the ncAA Kit Test]] | [[File:10-14-14 big experiment test tubes.png|450px|thumb|left| Preparation for the ncAA Kit Test]] | ||
[[File:RFP-GFP Controls 10-14-15.png|200px|thumb|right| A picture showing culture with or without IPTG. Without IPTG, there is no induction of GFP (left). With IPTG, strong fluorescence is easily seen (right).]] | [[File:RFP-GFP Controls 10-14-15.png|200px|thumb|right| A picture showing culture with or without IPTG. Without IPTG, there is no induction of GFP (left). With IPTG, strong fluorescence is easily seen (right).]] | ||
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=Results and Data= | =Results and Data= |
Revision as of 01:07, 17 October 2014
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