Encyclopedia of Experiments
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Encyclopedia of Experiments Neurowissenschaften
Isolating Murine Primary Oligodendrocytes Using Immunomagnetic Beads

Isolating Murine Primary Oligodendrocytes Using Immunomagnetic Beads

Transkript

After counting, centrifuge the cells again, and resuspend the pellet in 90 microliters of fresh magnetic cell-sorting buffer per 1 x 107 cells. Next, add 10 microliters of anti-O4 beads per 1 x 107 cells, and mix the cell solution with gentle flicking. After 15 minutes at 4 degrees Celsius, with gentle flicking, every 5 minutes, gently add 2 milliliters of magnetic cell-sorting buffer per 1 x 107 cells for a wash by centrifugation, and discard the supernatant by careful vacuum aspiration.

Resuspend the pellet in 500 microliters of fresh magnetic cell-sorting buffer for every 1 x 107 cells and place an appropriately-sized magnetic bead-sorting column into its corresponding magnetic separator. Place a 40-micron strainer onto the column and pre-rinse the strainer with 3 milliliters of magnetic cell-sorting buffer, letting the buffer run through the column without letting the column dry. Add the cells to the strainer, followed by a 1-milliliter wash with magnetic cell-sorting buffer.

Wash the column three times with 3 milliliters of magnetic cell-sorting buffer per wash, and one time with oligodendrocyte proliferation medium. Then, transfer the column into a 15-milliliter tube and use the plunger to immediately flush 5 milliliters of fresh oligodendrocyte proliferation medium through the column.

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