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Measurement Standard

⇐ Main Page

⇐ Measurements

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

HeLa, EGPF	HeLa, EBFP2	HeLa, EGPF and EBFP2	HeLa, EGPF and EBFP2 1:10
HEK T-REx, EGFP	HEK T-REx, EBFP2	HEK T-REx, EGPF and EBFP2	HEK T-REx, EGPF and EBFP2 1:10

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)

⇓ September

⇐ Main Page

⇐ Measurements

⇑ August

02/09/2010

seeding 1 96-well plate with all different cell lines we have (HelaP4, Hek293T and Huh7) for testing fluorescent measurement:
- purpose is to set up plate reader (TECAN), FACS and microscope and test whether it is possible to distinguish between GFP and BFP expression
- problem: forgot to coat the plate, therefore cells did not attach

03/09/2010

File:HeLa pilot GFP BFP2.jpg

FACS pilot experiment of EGFP and EBFP2 expression in Hela P4 cells

File:Huh7 pilot GFP BFP2.jpg

FACS pilot experiment of EGFP and EBFP2 expression in Hek T-Rex cells

File:HEK pilot GFP BFP2.jpg

Tecan pilot experiment of EBFP2 and EGFP expression with in Hela P4 cells‎‎

File:HEK TREx pilot GFP BFP2.jpg

Tecan pilot experiment of EBFP2 and EGFP expression with in Hek T-Rex cells‎‎

transfection of cells for fluorescent measurement (EGFP and EBFP2):

set-up of the plate:
- non-transfected cell line
- each cell line transfected with EGFP control plasmid
- each cell line transfected with EBFP2 control plasmid
- each cell line double-transfected with EGFP and EBFP2 control plasmids
- Results:
  - too little cells have been plated
  - Huh7 cells are hard to transfect
  - expression of EBFP2 is much lower than expression of EGFP

04/09/2010

seeding 1 96-well plate with all different cell lines we have (HelaP4, Hek293T and Huh7) for testing fluorescent measurement:
- purpose is to set up plate reader (TECAN), FACS and microscope and test whether it is possible to distinguish between GFP and BFP expression

05/09/2010

transfection of cells for fluorescent measurement (EGFP and EBFP2):
set-up of the plate:
- non-transfected cell line
- each cell line transfected with EGFP control plasmid
- each cell line transfected with EBFP2 control plasmid
- each cell line double-transfected with EGFP and EBFP2 control plasmids

06/09/2010

TECAN and FACS pilot measurements of cells transfected with EGFP and EBFP2

07/09/2010

seeding and transfection of HeLa and HEK cells for pilot microscopy measurements:

09/09/2010

pilot microscopy measurements:

20/09/2010

seeding 2 96-well plates with 5000 cells each well:
- test whether tuning construct is properly expressing firefly and renilla luciferase and thereby testing whether every part is functional

21/09/2010

transfection of both 96-well plates with K1-K8:
- transfect 50ng of each construct
- check for promoter strength and functionality of the constructs

22/09/2010

File:22092010promoters.jpg

relative expression units(REU) of firefly luciferase compared to renilla luciferase of the different tuning consstructs without any binding sites for the expressed shRNA10

File:22092010promoters2.jpg

comparison of REU of firefly to renilla luciferase in the different cell lines

dual luciferase assay on the 2 96-well plates:
- all constructs are functional as firefly and renilla luciferase are expressed
- transfection of construct into Hek t-Rex cells reveals that the CMVTetO2 (construct K4) is also functional as the expression of firefly to renilla counts is nearly zero

23/09/2010

dual luciferase assay

File:23092010promoters.jpg

500px

File:23092010promoters2.jpg