Notebook
- Our team pushed forward an experiment while making trial and error every day.
Creating parts of Tar methylation region
- Date:8/9
- Colony PCR
- →Reflection:We Took E.coli too many.You should take less E.coli.
- →Reflection:The number of cycles was less.So,We increased The number of cycles in 8/11.(50 cycles)
- Date:8/11
- The purified DNA
- →Reflection:Band was less.
- PCR Product
- Date:8/13 Confirmed of electrophoresis by PCR product and Ligation of the TA vector
- Date:8/14 Transformation
- Date:8/25 Miniprep
- Date:9/5 Miniprep,Nanodrop
- Date:9/6 Miniprep,PCR,Electrophoresis
- Date:9/10 Colony PCR,c,Ligation,Miniprep
- Date:9/11 Primer design
- Date:9/12 Miniprep,Ligation
- Date:9/13 Electrophoresis,Refinement of DNA
- Date:9/14 Colony PCR
- Date:9/15 Ligation
- Date:9/16 PCR,Ligation
- Date:9/17 PCR,Ligation
- Date:9/19 Ligation
- Date:9/20 Enzyme inactivation,Ligation
- Date:9/22 Transformation,Colony PCR,Electrophoresis,Miniprep
- Date:9/23 Colony PCR,Electrophoresis,Streak
- Date:9/25 Colony PCR
Creating parts of azurin
- Date:8/16
- Colony PCR
- Ligation
- Date:8/18 Colony PCR
- Date:8/20 DNA extraction and purification of P.aeruginosa
- Date:9/3 Ligation,Transformation,PCR,Nanodrop
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