Revised protocol for establishing a mammary cell line from tumors
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Revised protocol for establishing a mammary cell line from tumors
Drench mouse in 70% ethanol, pin and dissect open
Sterile dissection of tumor- leave some behind to use in histology
Place tumor in small culture dish
Weigh tumor in dish (empty dish weighs 2.8g)
Cover tumor with DMEM
Dissect remainder of mouse in non-sterile conditions (usual protocol). Include samples of tumor tissue in formalin and liq N2.
Prepare trypsin mix to digest tumor:
5 ml trypsin stock in 50 ml tube and add HANKs to 50 ml total vol (1x trypsin)
Mince tumor in culture dish using sterile scalpels until in cubes approx. 1mm3
Place minced tumor into 50 ml tube with 25 ml of trypsin mix. Add 1 drop DNAse. (NB. Depending on size of tumor might want to put into 2 tubes of 25 ml)
Shake tube(s) horizontallly at 37deg 60 rpm.
Observe at 15 min shaking
Observe at 30 min shaking ― retrieve?
If DNA has formed big blob of debris, add large amount (? 0.5 ml) DNAse to the blob and break it up with pipetting (10 ml pipette and / or pasteur).
Once blob sufficiently broken up, combine with remainder of cell mixture and filter through sterile gauze into sterile 50 ml tube.
Add equal volume of DMEM to cells to stop trypsin
Centrifuge 800 rpm 5 min
Decant supernatent
Resuspend pellet in 10 ml MEGM
Count cells
Prepare ECM gel:
Thaw ECM in room temp water then keep on ice
Chill few ml MEGM in 50 ml tube on ice
Chill 6 well plate on ice
Mix 1.5 ml ECM with 1.5 ml MEGM and keep mixture on ice
Pipette 600ul of mixture into the bottom of the 6 well plate ― 4 wells
Allow to gel at room temp in hood
Try approx 1 million cells per well (x2)
Also 2 million cells per well (x2)
Calculate volumes of cells needed for these numbers. Dilute in prechilled MEGM to 1 ml of appropriate concentration cells
Add 1 ml of ECM to cell mixes and mix ― keep chilled.
Pipette 1 ml of cells/MEGM/ECM mix to each well and mark the amount of cells added.
Allow to gel at room temp in hood
Cover with 1 ml MEGM when gelled
Incubator
Remainder of cells into 100 mm plates:
If possible set up 4 culture dishes MEGM x2
1 MEGM: 2 KGM
(One MEGM is for immunostaining; one 1 MEGM: 2 KGM will be changed to KGM only once cells have stuck down.)
