Results and Discussion:
Device 1 from Plate 7 was problematic to transform. We obtained no colonies after trying several times chemical transformation and electroporation, so we think there was some problem with that specific well. Then, we used the Device 1 from Plate 6, and we obtained several colonies that we could use for the InterLab. Later, we found that in the Registry of Standard Biological Parts website, it is stated that Device 1 is a complicated sample, so this could mean that there is some inherent problem with the device itself.
Most devices showed a similar growth behavior except Device 1, which had the lowest growth rate. In terms of fluorescence, the Device 2 produced the highest amount of fluorescence, even more than the positive control, followed by Device 4. The Device 3 and 6 produced no fluorescence. Device 1 and 5 produced very little fluorescence after 6 hours.
Since all the transformed bacteria showed very similar growth patterns across the devices, the lack of fluorescence can be attributed to a problem in the device itself or a transformation problem.
Regarding the plate reader measurements, bubble formation was problematic because it led to wrong measurements or outliers in our data. We solved this by checking for bubbles before measuring and we set the plate reader to lightly shake the plate while measuring the data. Also, we did three measurements per plate to minimize the outliers.
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