Illinois/1 July 2009
From 2009.igem.org
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July 1
sRNA Library
We re-did the PCR's, of the four sRNA's that didn't work. We also began a digestion of the two sRNA's and each of their target sequences.
The gel we ran after the PCR showed no bands. The gel we ran after the digestions showed strong bands, and we performed a gel extraction to purify the products. However the DNA concentrations we obtained from using the nanodrop were unusable.