IGEM:PKU Beijing/2009/Notebook/AND Gate 1/Output/2009/06/24/Shan Shen

10:50 Miniprep the plasmids containing T7 promoter, standard parts 1-12M and 1-12O. 1-12M: medium rbs + GFP coding gene + terminator 1-12O: strong rbs + GFP coding gene + terminator 12:30 Digest the plasmids of T7 promoter, 1-12M and 1-12O Digestion System for plasmids of T7 promoter:50μL Digestion System for plasmids of 1-12M and 1-12O: 50μL

12:50 Start to digest 14:20 Add CIAP into the system of vector digestion. 15:20 Electrophoresis to recycle the vectors and inserts of digestion. The order of the samples: marker, plasimid control of T7 promoter, T7 promoter, 1-12M, 1-12O. Results: Recycle the fragments (vector) of T7 promoter and the inserts of 1-12M, 1-12O. The fragment of T7 promoter is weird, for the linear plasmids ran even faster than the round ones. Decide to do some controls and tests