C2C12 cell transfection with FuGene: Difference between revisions
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''2 x 6cm dishes with C2C12 cells'' | ''2 x 6cm dishes with C2C12 cells'' | ||
== | == Material == | ||
{| class="wikitable" | {| class="wikitable" | ||
!style="width: | !style="width: 10px" | Day | ||
!style="width: 590px" | Material | |||
!style="width: | |||
|- | |- | ||
| | |first | ||
| 2x 6cm dishes | |||
75 cm2 flask | 75 cm2 flask | ||
C2C12 cells in a 75 cm2 flask | C2C12 cells in a 75 cm2 flask | ||
Line 19: | Line 16: | ||
Neubauer chamber for counting the cells | Neubauer chamber for counting the cells | ||
Pipettes and tips | Pipettes and tips | ||
|- | |||
|second | |||
| | |||
DMEM (4500mg/l Glucose) | DMEM (4500mg/l Glucose) | ||
FuGene Transfection reagent | FuGene Transfection reagent | ||
Line 26: | Line 25: | ||
high serum media for C2C12 | high serum media for C2C12 | ||
pipettes and tips | pipettes and tips | ||
|- | |||
|third | |||
| | |||
Fresh prepared non-serum-T.i.- media | Fresh prepared non-serum-T.i.- media | ||
PBS | PBS | ||
|- | |||
|fourth | |||
| | |||
PBS | PBS | ||
Fresh prepared 2% Horse Serum- low serum | Fresh prepared 2% Horse Serum- low serum | ||
|} | |||
== Procedure == | |||
{| class="wikitable" | |||
!style="width: 10px" | Day | |||
!style="width: 590px" | Procedure | |||
|- | |||
|first | |||
| | |||
# wash the cells with 5 ml PBS | |||
# add 2 ml of TE to the cells and incubate them for 2 min at 37ºC | |||
# during this time: label the new flask and the 2 6cm dishes with the name and the passage number of the cells and the date and fill in the flask 15 ml of new media | |||
# stop the TE with the 5 ml of the HS – media | |||
# transfer the cell suspension into the 15 ml FALCON tube | |||
# centrifuge the cells: 1000xg for 3 min at +4ºC | |||
# remove the old media and dissolve the cell pellet in a few ml of fresh media (the amount of media correlates with the pellet- the cells should be not to dense or to diluted for the counting – general 3 ml are fine for a pellet of one 75cm2 flask of C2C12) | |||
# prepare the Neubauer camber (put the cover slip over the chamber and move it a little bit till you can see the Newton’s rings!!! – this is important for the calculation!!) | |||
# fill between the camber and the cover slip around 40 ml of cell suspension | |||
# count the cells under the scope (all 4 corner crosses - each corner cross has 16 little crosses)- count the both main crosses | |||
# to calculate the number of cells which are in (f.ex. in total 3mls) suspension, calculate at first the average of the 8 crosses, than multiply the average with 104 (the number of cells in 1 ml (!) of suspension) and than multiply this with the amount of ml of the suspension (f.ex. 3) – this is the total number of cells | |||
# pipette in each 6 cm dish 350.000 cells 9next day: use this for transfection) and in the flask 1:30 | |||
# 6 cm dishes: fill up to total 5 ml with fresh media | |||
# move the dishes like a cross that the cells are homogenized in the dish | |||
# let them grow at 37ºC, 10% CO2 | |||
|- | |||
|second | |||
| | |||
- | # FuGene transfection reagent (stored at –20ºC) and plasmid on ice | ||
# For 2 transfections: | |||
o 1) per transfection: 1µg plasmid in 40 µl DMEM | |||
o –for 2 transfections: 2µg plasmid in 80 µl | |||
o DMEM | |||
o pipette this in one 1.5ml eppendorf tube together | |||
2) per transfection: 6µl of FuGene transfection reagent into 154 | |||
o 1) per transfection: 1µg plasmid in 40 µl DMEM | |||
o –for 2 transfections: 2µg plasmid in 80 µl | |||
o DMEM | |||
o pipette this in one 1.5ml eppendorf tube together | |||
2) per transfection: 6µl of FuGene transfection reagent into 154 | |||
µl DMEM (total volume: 160µl) into a second 1.5ml eppendorf tube | µl DMEM (total volume: 160µl) into a second 1.5ml eppendorf tube | ||
-for 2.5 transfections: 15 µl FuGene transfection reagent in | -for 2.5 transfections: 15 µl FuGene transfection reagent in | ||
385 µl DMEM (in tube one should be now 400µl-> 200µl per | 385 µl DMEM (in tube one should be now 400µl-> 200µl per | ||
transformation) | transformation) | ||
[pipette at first the DMEM into the second tube and | |||
than into the DMEM the FuGene! | than into the DMEM the FuGene!] | ||
3) pipette from the second tube (FuGene-DMEM-Mix) 320 µl of the Mix into the first tube (DNA-DMEM-Mix) | 3) pipette from the second tube (FuGene-DMEM-Mix) 320 µl of the Mix into the first tube (DNA-DMEM-Mix) | ||
4) incubate the FuGene-DNA-DMEM-Mix for 15 min at RT | 4) incubate the FuGene-DNA-DMEM-Mix for 15 min at RT | ||
# during this time: remove the media from the cells and add in each dish 1.8 ml of DMEM- put this for the rest of the incubation time at 37ºC (incubator) | |||
# after the 15 min take the cells put from the incubator and drop wise pipette into each dish 200µl of Fugene-DNA-DMEM-Mix | |||
# incubate this for one hour at 37ºC (incubator) | |||
# after this: ADD 4 ml of high serum media to each dish | |||
# dishes back in the incubator (37ºC, 10%CO2) | |||
|- | |||
|third | |||
| | |||
# if all wash fine, than the cells should be now confluent | |||
# if this is the case: remove the media, wash the cells twice with PBS and add 5 ml of Non-serum-T.i.-medium to each dish | |||
|- | |||
|fourth | |||
| | |||
# remove the media and wash the cells twice with PBS | |||
# add 5 ml of 2% HS-LS to each dish | |||
|} |
Latest revision as of 14:32, 8 June 2015
2 x 6cm dishes with C2C12 cells
Material
Day | Material |
---|---|
first | 2x 6cm dishes
75 cm2 flask C2C12 cells in a 75 cm2 flask 15 ml FALCON tubes High serum media for C2C12 TE in PBS PBS Neubauer chamber for counting the cells Pipettes and tips |
second |
DMEM (4500mg/l Glucose) FuGene Transfection reagent the plasmid which should be transfected 1.5 ml eppendorf tubes high serum media for C2C12 pipettes and tips |
third |
Fresh prepared non-serum-T.i.- media PBS |
fourth |
PBS Fresh prepared 2% Horse Serum- low serum |
Procedure
Day | Procedure |
---|---|
first |
|
second |
o 1) per transfection: 1µg plasmid in 40 µl DMEM o –for 2 transfections: 2µg plasmid in 80 µl o DMEM o pipette this in one 1.5ml eppendorf tube together 2) per transfection: 6µl of FuGene transfection reagent into 154 µl DMEM (total volume: 160µl) into a second 1.5ml eppendorf tube -for 2.5 transfections: 15 µl FuGene transfection reagent in 385 µl DMEM (in tube one should be now 400µl-> 200µl per transformation) [pipette at first the DMEM into the second tube and than into the DMEM the FuGene!] 3) pipette from the second tube (FuGene-DMEM-Mix) 320 µl of the Mix into the first tube (DNA-DMEM-Mix) 4) incubate the FuGene-DNA-DMEM-Mix for 15 min at RT
|
third |
|
fourth |
|