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From 2010.igem.org

Contents 1 08/08/2010 2 09/08/2010 3 10/08/2010 4 25/08/2010 5 26/08/2010 6 27/08/2010

08/08/2010

seeding cells for test measurements - 96 well plate for plate-reader and FACS

• cells were grown in DMEM 10%FBS with phenol red
• washed with PBS
• trypsinised (2 ml trypsin)
• 5ml of OptiMEM media (no FBS) added
• counted cells: HeLa 3.8*10^6 cells/ml, HEK 3.3*10^6 cells/ml, HEK T-Rex 1.5*10^6 cells/ml, Huh7 0.8*10^6 cells/ml
• seeded 5000 and 2500 cells/well as on the scheme 96well plate 080810.jpg
• media: DMEM +L-Glu +PenStrep +10%FBS, OptiMEM +PenStrep, OptiMEM +PenStrep +2%FBS
• in all wells where T-Rex cells were seeded zeocin and blasticin were added, in wells with Huh7 cells - non essential amino acids

-> cells did not adhere well, coat plate with poly-L-lysine and repeat

09/08/2010

seeding and transfecting cells for microscopy test measurements

• add 0.6ul FuGENE reagent to 20ul of OptiMEM
• mix and incubate 5' at RT
• add 0.2ug DNA
• mix and incubate 15' at RT
• add DNA-FuGENE solution to 10 000 cells (400ul)
• mix and incubate 10' 37degC 300rpm (shaker for 15ml falcon tubes is in the cell culture room at 3rd floor)
• transfere cells to the plate
• grow 48h

10/08/2010

coating plates with poly-L-lysine

• add 15ul of poly-L-lysine solution to each well (make sure whole surface is covered with solution)
• leave for 30' in the incubator
• remove poly-L-lysine solution
• wash once with PBS

new 96-well plate was prepared (wells 2500 cells Huh7 are contaminated with HeLa) like previously

25/08/2010

seeding cells for pilot FACS and Tecan measurements (96-well plate)

26/08/2010

transfection - 96-well plate

27/08/2010

pilot FACS and Tecan measurements (96-well plate)