Team:Nevada/Week 15
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Contents |
August 27
- Joe: fusion and transformation
- Michelle:
- Pellet large scale expression to prepare for purification of M2-BL21 glycerol stock
- + LB AMP-CM.
LJustin and Dafne:
- Determine optimal Imidazole concentration to utilize in Ni-column purification
- Create 12 mM, 14 mM, 16 mM Imidazole binding buffers
- Three seperate protein expressions were carried out (as done above)
- Each pellet was suspended in one of the binding buffers and then the cells were lysed using the sonicator (as :::done before)
- The supernatant of each different binding buffer was run through the Ni-column
- Jeremiah & Chris:
- Transformation failed
- Set up phusion for TET plasmid
- Ligate the phusion products (TET and TBP+)
August 28
- Joe:
- Redigestion of RFPEP-R by DpnI
- PCR of SBP-R, RFP-R using longamp
- Michelle:
- Purification of large scale expression of M2-BL21 glycerol stock + LB AMP-CM using a Nickel column.
- Conducted SDS-PAGE Coomassie and Western Transfer Blot protocol, which continued until tomorrow.
- Justin and Dafne:
- Western blot analysis of above protein purification
- Western blot analysis was uninspiring, indicating the concentration change did not effect purification
- Jeremiah & Chris:
- Run ligation on a gel (gel #176)
- Gel showed no ligation occurred
- Phusion PCR the TET plasmid and TBP+ gene (Long Amp Taq)
- Ligate the phusion products
- Transform into TOP 10 cells
August 29
- Michelle:
- SDS-PAGE Coomassie staining of gel followed by desalting of protein at ~30kDa, which was successful.
August 30
- Joe:
- PCR clean up - gel 173 good
- Transform, plate on AMP
- Michelle:
- Develop Western Transfer Blot of purified large scale expression of M2-BL21 glycerol stock + LB AMP-CM.
- Modified ELISA assay using starch and testing with iodine to check the presence of starch in wells. Purified :::SBP-LRP also tested with Starch-ELISA.
August 31
- Joe:
- Colony PCR of RFPEP-R