Isolate or Deplete CD19+ B Cells - Whole Blood, Buffy Coat, MNC Suspensions

Isolate or deplete CD19⁺ B cells directly from whole blood, buffy coat or MNC suspensions. For rapid and consistent results in protein or gene expression analysis, lyse the cells while they are still attached to the beads and directly process for further molecular analysis.

Note: To detach the Dynabeads from the isolated cells, use DETACHaBEAD® CD19 (not supplied).

Principle of Isolation

Dynabeads are mixed with the sample in a tube. The Dynabeads will bind to the target cells during a short incubation, and then the bead-bound cells are separated by a magnet.

• Positive isolation – discard the supernatant and use the bead-bound cells for downstream applications (e.g. molecular analysis or cell culture).
• Depletion – discard the bead-bound cells and use the remaining, untouched cells for any application.

Description of Materials

Dynabeads CD19 are uniform, superparamagnetic polystyrene beads (4.5 μm diameter) coated with a monoclonal antibody specific for the CD19 membrane antigen.

Materials Supplied

• 5 ml Dynabeads CD19 pan B 4 x 10⁸beads/ml in phosphate buffered saline (PBS), pH 7.4, containing 0.1% bovine serum albumin (BSA) and 0.02% sodium azide (NaN₃).
• This product can be used to process up to 5 x 10⁹ cells.

Additional Materials Required

• Magnet (Dynal MPC™): See www.lifetechnologies.com/magnets-selection for magnet recommendations.
• Mixer allowing both tilting and rotation.
• Buffer 1: PBS (without Ca²⁺ and Mg²⁺) w/0.1% BSA and 2 mM EDTA, pH 7.4.
• Optional: DETACHaBEAD CD19 (Cat. no. 125.06D)

• Use a mixer that tilts and rotates the tubes to ensure Dynabeads do not settle at the bottom of the tube.
• When incubating Dynabeads and cells, the incubation temperature must be 2 - 8°C to reduce phagocytic activity and other metabolic processes.
• Never use less than 25 μl Dynabeads per ml cell sample and at least 4 Dynabeads per target cell.

1. Add Dynabeads to the prepared sample according to table 1.
   
   
2. Incubate for 20 min (positive isolation) or 30 min (depletion) at 2 - 8°C with gentle tilting and rotation.
   
   
3. Place the tube in a magnet for 2 min.
   
   
4. Depletion: Transfer the supernatant containing the unbound cells to a fresh tube for further experiments.
   
   
5. Positive isolation: Discard the supernatant and gently wash the bead-bound cells 4 times, using the following procedure:

   
               i) Add 1 ml Buffer 1 per 1 x 10⁷Dynabeads.
   
               ii) Place the tube in the magnet for 1 min and discard the supernatant.
   

6. Resuspend the cells in buffer/medium for downstream application. For molecular studies, lyse cells while still attached to the beads and transfer supernatant to a new tube for protein or gene expression analysis.

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