200,000 tumor cells or peptide-pulsed 293T-A1 cells were seeded in each well of 96-well plate overnight. Next day, 200,000 MAGE-A3-specific TCR-transduced human primary cells were mixed with 1:100 anti-CD107a-PE (clone H4A3, BioLegend) and 1:1000 brefeldin A, and then added to each well. Coculture was done for 6 hours at 37 °C, 5% CO2. After 6 hours, the plate was stained with anti-CD8-BV421 (clone RPA-T8, BD Biosciences), anti-Vβ5.1-APC. Then the plate was fixed with IC fixation and permeabilized by permeabilization buffer. The plate was further stained with anti-IFN-γ-BV605 (clone B27, BioLegend) and anti-TNF-PE-Cy7 clone MAb11, BioLegend) on ice for 30 min. The plate was then washed and analyzed by CytoFLEX.
Anti cd107a pe clone h4a3
Manufactured by BioLegend
Anti-CD107a-PE (clone H4A3) is a fluorescently-labeled monoclonal antibody that specifically binds to the CD107a (also known as LAMP-1) surface antigen. CD107a is a lysosome-associated membrane protein that is expressed on the cell surface during degranulation, making it a useful marker for the identification of cytotoxic cell populations.
Automatically generated - may contain errors
Lab products found in correlation
Nkg2d pe, by BioLegend (1 mentions)
Clone mopc 21, by BioLegend (1 mentions)
Zombie nir viability dye, by BioLegend (1 mentions)
Facs lsrfortessa x 20 flow cytometer, by BD (1 mentions)
Nkp44 apc, by BioLegend (1 mentions)
Nkp46 percp cy5, by BioLegend (1 mentions)
Nkp30 af647, by BioLegend (1 mentions)
Lfa 1 pe, by BioLegend (1 mentions)
Anti cd56 af488 mab clone hcd56, by BioLegend (1 mentions)
Golgiplug, by BD (1 mentions)
Monensin, by BioLegend (1 mentions)
2 protocols using anti cd107a pe clone h4a3
1
Evaluating MAGE-A3-specific TCR Activity
2
Assessing NK Cell Degranulation
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To assess degranulation, NK cells were co-incubated with opsonized target cell lines in the presence of GolgiPlug (1/1000 dilution, BD Biosciences), monensin (1/1000 dilution, Biolegend) and anti-CD107a PE mAb (clone H4A3, BD biosciences) or an isotype-matched control (PE-IgG1κ; clone MOPC-21, BD) for 4 h at 37°C. After incubation, cells were washed and stained with Zombie NIR viability dye (Biolegend), anti-CD56-AF488 mAb (clone HCD56, Biolegend), anti-CD107a-PE (clone H4A3) and anti-CD16-AF647 (clone; B.731, Biolegend) (42 (link)). To assess expression of other proteins, NK cells were co-incubated with opsonized target cell lines for 4 h, then washed and stained with Zombie NIR viability dye (Biolegend) and LFA-1-PE (Clone M24), NKp46-PercP-Cy5.5 (Clone 9E2) and NKp44-APC (Clone P44-8) or NKp30-AF647 (Clone P30-15) and NKG2D-PE (Clone 1D11, all from Biolegend). Isotype-matched control mAbs were also used accordingly (mouse IgG1 isotype control; clone MOPC-21, Biolegend). Finally, cells were fixed in 2% PFA/PBS and staining was assessed using a BD FACS LSRFortessa™ X-20 flow cytometer and analyzed by FlowJo V10 software (BD Biosciences). The gating strategy used for all flow cytometry assays is shown in Supplementary Figure 5 .
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