Virginia/8 July 2008

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Goals

Prepare overnight broth of single successful colony of Promoter + RBS transformation
Plate Screening plasmid (psb1a10) when it arrives from iGem
Try again with ligation of RFP and GFP enzyme cut DNA
Transform this ligation and pray that it grows in the incubator
Run a gel of linearized and cut DNA of BP1 and terminator assembly to verify transformation
Begin ligation of standard RBS with BP1 gene to begin parallel assembly of our final operon

Notes

Maxiprepped bba_B0015 and bba_B0034 smell strongly of alcohol, we are dubious of the content of the prepared DNA

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