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Dans cet article

  • Overview
  • Protocole
  • Déclarations de divulgation
  • matériels

Overview

This video demonstrates T cell isolation from peripheral blood mononuclear cells (PBMCs) using the functionalized buoyancy-activated cell sorting (BACS) technology. The isolation technique involves the positive selection of CD3+ T cells by labeling the cells with biotinylated anti-CD3 antibodies and separating the antibody-bound cells using streptavidin-bound microbubbles.

Protocole

1. Isolation of T cells with microbubbles using positive selection

NOTE: This protocol details a small-scale CD3+ positive selection approach using SAMBs.

  1. Incubate 3 x 108 commercially obtained PBMCs in 2.5 mL of separation buffer with biotinylated anti-CD3 (OKT3) antibody at a concentration of 25 ng of antibody per 1 million cells (25 ng/M). Gently mix by pipetting up and down, and incubate at room temperature for 10 min.
  2. Add streptavidin microbubbles (SAMBs) at a ratio of 0.5 (SAMB quantity):1 (cell quantity) according to the manufacturer's reported SAMB concentration.
  3. Mix using a commercial end-over-end (EOE) rotator at 20 rpm for 10-15 min at room temperature. Centrifuge for 5 min at 400 x g at room temperature.
  4. After centrifugation, the positively selected cells will be at the top of the suspension with the SAMBs. The remaining non-selected cells will be in the cell pellet at the bottom of the tube. Using a 9in glass pipette, insert the tip below the bubble-cell layer to the bottom of the tube, aspirate the cell pellet and subnatant with an electronic pipette, and transfer them to a new tube.

Déclarations de divulgation

No conflicts of interest declared.

matériels

NameCompanyCatalog NumberComments
Biotin anti-human CD3 (OKT3) AntibodyBiolegend317320
LeukopakBioIVTHUMANLMX100-0001129
Normal Human PBMCsBioIVTHUMANHLPB-0002562
Streptavidin Microbubble Kit (includes Akadeum's separation buffer)Akadeum11110-000

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