Part:BBa_K1111002:Experience
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how you used this part and how it worked out.
Applications of BBa_K1111002
We wanted to test if the promoter that we cloned into the plasmid really can be induced upon external acidification. In order to do that, we transformed bacteria with it, incubated them at different pH and then measured their GFP expression using a plate reader.
Gibson Assembly
We used Gibson Assembly to insert the Cad promoter into the pSB1C3 Backbone. We used the biobrick BBa_I746908 where we remove the Arac promoter but left the superfolded GFP. This way, the latter was under control of our Cad promoter.
Sequencing
The sequencing result showed that there were no mutations in the insert
OD Measurements
We transformed cell with our plasmid and then measured their OD in different media with different pHs. We compared this data with the Fluorescence measurements and were able to conclude that the reason why GFP is not expressed at low pH is that the bacteria are actually dying in these two media
Measuring Fluorescence with a PlateReader
We wanted to know if the promoters were indeed induced at low pH. For this we let the bacteria grow in differenly buffered media in aplate reader and the measured their Fluorescence.
Observing Fluorescence under the Microscope
We wanted to induce GFP expression in our bacteria by adding different buffers to the media. We then let them grow for a while and then looked at them under the microscope to see if they were expressing GFP or not. We compared their fluorescence with another biobrick we made in which we put a constitutive promoter in fron of superfolded GFP as a qualitative measure.
User Reviews
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