Team:Groningen/Labwork/30 July 2013
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Revision as of 13:15, 30 July 2013 by SanderWallert (Talk | contribs)
Mirjam
Started gel extraction for the restricted backbone+promoter, RFP and eYFP. RFP and eYFP are dissolved in 30µl elution buffer, to get a higher concentrationRun a 0.8% agarose gel to examine the restriction. Gel revealed only a very small band for RFP.
Did a nanodrop on the samples to examine their concentration. Concentration of the backbone is 0.8 ng/µl, RFP 6.4 ng/µl and eYFP 2.4 ng/µl.
Did a new restriction digestion for BBa_k823823 + LacI with EcoRI and PstI, using 500 and 250ng.
Chaline & Mirjam
Did a restriction digestion for eYFP with EcoRI and PstI using 200ng.Run the samples of restricted eYFP and the backbone on gel for gel extraction. But the concentration of the eYFP looks again very low. For all samples the band is extracted from gel. Concentration is measured and again the concentration seems way to low, for what we expected. The samples are run on gel to determine if the number of bp is the expected one. No bands are seen on gel. But trusted the concentrations and continued with a ligation reaction.
Transformation to E. coli with half of the ligation of the backbone with eYFP and the ligation of the backbone with RFP. Also made a new transformation to obtain more RFP and eYFP.
Claudio
The transformation of BBa_E0840 and BBa_E0240 worked because cells grew in LB + chloramphenicol. The inoculation of mKate2 worked.Plasmids are isolated from the inoculations.
BBa_K823023 + lacI, BBa_E0840, BBa_E0240 and mKate2 are digested with XbaI and PstI.
Sander
did a miniprep for BBa_E0240, BBa_E0840 and mKate2, DNA concentations to low.