Team:TUDelft/4 August 2009
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Revision as of 12:58, 10 September 2009
Lab Notebook
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4 August 2009
Orr
Prepared some LB Agar medium, and continued with writing the code for the software constructing lock and key sequences for the cascade delay device.
Calin
Trimethoprim finally arrived. Made trimethoprim 4 x 1 mL eppendorfs stock solution of 10 mg/mL using DMSO solution.
Transformed the first two ligations (CA & CB).
Made two R751 plates with 2xTRI.
Made a 5 mL tube of pTet-GFP with AMP and another 5 mL tube of R751 with TRI.
Tim Weenink
none of yesterdays transformations worked. To find out why, a gel was prepared with the DNA fragments that were used. Also, a PCR reaction of the all the colonies from !D transformation was done. For this the primers I-SceI forward and VR were used. Thirdly, *S, *T, *E, *G, *P PCR products were purified. This was done because it was found that adding 10µl of PCR reaction mix directly to the restriction mix will cuase star activity.
Results of the gel are on next days page.
results of the purification:
Part | DNA concentration | 260/280 | 260/230 |
BBa_B0015 | 9.5 | 2.15 | 1.96 |
BBa_R0040 | 58.2 | 1.56 | 0.66 |
BBa_K145201 | 14.5 | 1.74 | 2.21 |
BBa_K142205 | 14.1 | 1.75 | 2.64 |
BBa_K142202 | 4.3 | 2.66 | 4.24 |