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  • 發布時間:2019-04-28 20:30 原文鏈接: SOFTAGARASSAYFORCOLONYFORMATION

    Note: All volumes are calculated to cater for four plates per point.

    Base Agar

    1. Melt 1% Agar (DNA grade) in microwave, cool to 40 in a waterbath. Warm 2X RPMI + 20% FCS to 40 in waterbath. Allow at least 30 minutes for temperature to equilibrate.

    2. Mix equal volumes of the two solutions to give 0.5% Agar + 1X RPMI + 10% FCS.

    3. Add 1.5ml/ 35 m Petri dish, allow to set. The plates can be stored at 4 for up to 1 week.

    Top Agar

    1. Melt 0.7% Agar (DNA grade agarose) in microwave, cool to 40 in a waterbath. (It is important not to exceed 40, otherwise cells will be killed). Also warm 2X RPMI + 20% FCS to the same temperature.

    2. Trypsinise cells and count. It is very important to have a positive control line (eg. ras transformed).

    3. You require 5,000 cells/plate, therefore you need 20,000/tube. Adjust cell count to 200,000 cells /ml.

    4. Add 0.1ml of cell suspension to 10ml yellow capped centrifuge tubes.

    5. Label 35mm petri dishes with base agar appropriately (it is a good idea to remove the plates from 4 about 30 minutes prior to plating to allow them to warm up to room temperature).

    6. For plating add 3ml 2X RPMI + 10% or 20% FCS and 3ml 0.7% Agar to a tube, mix gently and add 1.5ml to each replicate plate (usually plate out in triplicate). NOTE: Only do one tube at a time so that agar does not set prematurely.

    7. Incubate assay at 37 in humidified incubator for 10 - 14 days.

    8. Stain plates with 0.5ml of 0.005% Crystal Violet for >1 hour, count colonies using a dissecting microscope.


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