Pe conjugated cd56

Analysis of cell surface–mobilized CD107a (degranulation assay) has been previously described [39 (link)]. Briefly, NK cells (50,000) were incubated either alone or with 721.221 target cells (50,000 cells), APC conjugated CD107a (BioLegend) and PE conjugated CD56 (BioLegend), for 2 hours in 37°C. Following incubation, CD107a expression was analyzed using flow cytometry.

Fluorescent‐conjugated anti‐human antibodies including fluorescein isothiocyanate (FITC)‐conjugated CD16 (clone: B73.1), phycoerythrin (PE)‐conjugated CD56 (5.1H11), Peridinin‐chlorophyll‐protein complex (PerCP)‐conjugated NKp44 (clone: P44‐8), Allophycocyanin (APC)‐conjugated CD3 (clone: OKT3), FITC‐conjugated CD3 (clone: OKT3), PerCP‐conjugated CD3 (clone: HIT3a), PerCp‐Cy5 conjugated CXCR3 (clone: G025H7), PerCp‐Cy5‐conjugated NKG2D (clone: 1D11), APC‐conjugated CD11b (clone: ICRF44), PerCP‐Cy5.5–conjugated CD27 (clone: M‐T271), PerCP‐Cy5.5‐conjugated perforin (clone: B‐D48), Alexa Fluor® 647‐conjugated granzyme B (clone: GB11), PerCP‐Cy5.5‐conjugated CD96 (clone: NK92.39) and their cognate isotype controls (all from Biolegend) as well as PerCP‐Cy5.5‐conjugated NKG2C (clone: 134591, R&D system) antibodies were used for immunophenotyping. Lysing solution (BD Biosciences) was used for removing the red blood cells. For washing, fixing, and cell permeabilizing, 1X phosphate buffer saline (PBS), 1% paraformaldehyde solution (Sigma), and 1X perm/wash solution (BD Biosciences) were used, respectively.