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NK cell survival mediated through the regulatory synapse with human DCs requires IL-15Rα
Fabienne Brilot, Till Strowig, Susanne M. Roberts, Frida Arrey, Christian Münz
Fabienne Brilot, Till Strowig, Susanne M. Roberts, Frida Arrey, Christian Münz
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Research Article Immunology

NK cell survival mediated through the regulatory synapse with human DCs requires IL-15Rα

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Abstract

DCs activate NK cells during innate immune responses to viral infections. However, the composition and kinetics of the immunological synapse mediating this interaction are largely unknown. Here, we report the rapid formation of an immunological synapse between human resting NK cells and mature DCs. Although inhibitory NK cell receptors were polarized to this synapse, where they are known to protect mature DCs from NK cell lysis, the NK cell also received activation signals that induced mobilization of intracellular calcium and CD69 upregulation. The high-affinity component of the receptor for IL-15, IL-15Rα, accumulated at the synapse center on NK cells, and blocking of IL-15Rα increased NK cell apoptosis and diminished NK cell survival during their interaction with DCs. Furthermore, IL-15Rα–deficient NK cells, obtained from donors with a history of infectious mononucleosis, showed diminished survival in culture with DCs. Synapse formation was required for IL-15Rα–mediated NK cell survival, because synapse disruption by adhesion molecule blocking decreased DC-induced NK cell survival. These results identify what we believe to be a novel regulatory NK cell synapse with hallmarks of spatially separated inhibitory and activating interactions at its center. We suggest that this synapse formation enables optimal NK cell activation by DCs during innate immune responses.

Authors

Fabienne Brilot, Till Strowig, Susanne M. Roberts, Frida Arrey, Christian Münz

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Figure 8

Blocking of IL-15Rα decreased NK cell survival and upregulated annexin V binding on both NK cell subpopulations.

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Blocking of IL-15Rα decreased NK cell survival and upregulated annexin V...
(A and B) Blood NK cells were purified and treated for 6 h with polyclonal anti–IL-15Rα or control goat IgG, and cocultured with poly(I:C)-matured DCs during 9 days, counted, stained, and analyzed by flow cytometry. Results are mean ± SD of (A) ratios of output to input of live NK cells normalized to controls or (B) absolute numbers of live cells compared with controls in at least 3 experiments ran in triplicate. *P < 0.001 versus control (NK + DC). NK cells were gated on size, 7AAD–, CD3–, CD16+/–, and CD56+. (C) Annexin V binding was analyzed with and without blocking of IL-15Rα. Representative data from at least 3 different experiments are shown. (D) Annexin V binding on the surface of both NK cell subsets was determined. Results are mean ± SD of mean fluorescence intensity (MFI) of annexin V staining. *P < 0.02 versus control (NK + DC). Data are representative of 3 experiments.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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