Difference between revisions of "Part:BBa K606041:Experience"
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= Characterization tRNA amber suppressor= | = Characterization tRNA amber suppressor= | ||
==Protocol== | ==Protocol== |
Revision as of 19:47, 19 October 2011
Characterization tRNA amber suppressor
Protocol
In order to characterize the tRNA amber suppressor, as well as the pHyperspank, a special part was made: Pveg-SpoVG-GFP amber-TT. A double transformation was done with minipreps of two plasmids of different antibiotic resistances : pSB1C3 holding the tRNA under the control of pHyperspank and pSB1AK3 holding the GFP with the amber codon under the control of a constitutive promotor. Two groups of cultures of each picked colony were made. One group was cultured in rich medium without IPTG whilst the other group was cultured in rich medium with IPTG (4mM in 10mL). A culture of the strain holding GFP amber alone was grown in parallel. The two tubes of each colony were compared along with the negative control (GFP amber alone). Cultures were then diluted for microscopy, glycerols, and future experiments. We used the following strains to characterize this system:
GFP amber Strain holding GFPmut3B, mutated with a single amber mutation under the control of the constitutive promotor Pveg, in the plasmid pSB1AK3 (AmpR).
tRNA amber suppressor Strain holding the tRNA amber suppressor, under the control of IPTG inducible strong promotor pHyperspank, in the plasmid pSB1C3 (CmR).
Double transformant Double transformant of the two previous constructs in their plasmids respectively. Two groups of cultures are grown: with or without IPTG.
Direct observation under fluorescence lamp and microscopy was used to characterize this system.
We have also characterised the pHyperSpank promoter, compatible with B.subtilis and which is used in this system.
Characterization of the tRNA biobrick (fluorescence lamp)
The cultures of strains having transformed both tRNA amber suppressor and GFP amber were strongly fluorescent, while the culture of the GFP amber alone as well as the culture of the colony without IPTG induction showed basal fluorescence.
Characterization of the tRNA biobrick (microscopy)
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