Frequently Asked Questions for Using Suspension Cells

07 Mar.,2024

 

    Frequently Asked Questions for Using Suspension Cells

  1. How do you culture suspension cells?

    For instructions on culturing suspension cells, look up your cell line at http://www.atcc.org/ and follow the guidelines.

  2. How do you make non-adherent cells (suspension cells) attach to plates?

    A simple trick is to replace your complete media containing 10% serum (usually fetal bovine serum) with the same media minus the serum. Then allow the cells to sediment, forming

    a monolayer of cells within 10 minutes. Caution: Although cells appear attached to the plates, they are relatively loosely attached; therefore, extreme caution is required during solution- changing steps.

  3. How do I know that I have a monolayer?

    Method #1 – Examine cells in the round bottom 96-well plates under a light microscope. The

    center of the wells should all have a small flat circular surface area where all the cells in that

    field are “in focus”. Moving the plane of focus up or down will cause cells to be “off focus”.

    Method #2 – Hold the round bottom 96-well plate under a light source. The monolayer should look opaque rather than transparent. Cells will not attach on top of the cell monolayer, so the opaqueness is due only to the monolayer.

  4. I cannot get a monolayer of cells. I get lots of spaces between cells. Is seeding 200,000 cells/well enough?

    Seeding 200,000 cells/well is more than enough to form a complete cell monolayer. It is necessary to allow the cells in serum-free media to sediment in the T75 flask (or other tissue culture plates) for approximately 30 minutes before counting cells using a hemacytometer.

    When cells in serum-free media are placed, for example, in a T7 tissue culture flask, a monolayer of cells will immediately begin to form on the bottom of the flask. This will dramatically decrease the number of cells in suspension that are available for plating. NOTE: Once a complete monolayer has formed on the plate, the rest of the cells will remain in suspension.

    Count these cells in suspension and the cells attached to the T75 flask can be discarded later.

    1.5 During my washing steps, cells are coming off the plates.

        1. Are you using the recommended round bottom 96-well plate (BD Bioscience, P/N 353077)?

          If no, cells will more easily detach from the flat bottom plates than the round bottom plates. The multi-channel pipettors will generate enough pressure when expelling liquid from the pipet to cause cell detachment when using flat bottom plates. Cells will detach even when pipetting down the sides of the wells.

          If yes, make sure you pipet down the sides of the wells and not directly onto the cells. If this

          doesn’t help, you may need to change your multi-channel pipettor because different brands of pipettors have different amount of pressure required to expel the liquid from the pipet. The recommended multi-channel pipettor is the 12-channel Finnpipette (Thermo Electron Corp,

          P/N 4610050).

        2. Are you shaking or rotating the plates at a moderate-to-high speed?

    If yes, gentler shaking/rotating is needed to prevent cells from detaching. Cells will detach. Set shaking or rotating speed to very low speed.

    If no, are you dumping the solutions straight from the plates? Dumping causes cells to detach. Either aspirate very slowly or manually pipet using the sides of the wells.

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