Abstract
The NK cell population is characterized by distinct NK cell subsets that respond differently to the various activating stimuli. For this reason, the determination of the optimal cytotoxic activation of the different NK cell subsets can be a crucial aspect to be exploited to counter cancer cells in oncologic patients. To evaluate how the triggering of different combination of activating receptors can affect the cytotoxic responses of different NK cell subsets, we developed a microbead-based degranulation assay. By using this new assay, we were able to detect CD107a+ degranulating NK cells even within the less cytotoxic subsets (i.e., resting CD56bright and unlicensed CD56dim NK cells), thus demonstrating its high sensitivity. Interestingly, signals delivered by the co-engagement of NKp46 with 2B4, but not with CD2 or DNAM-1, strongly cooperate to enhance degranulation on both licensed and unlicensed CD56dim NK cells. Of note, 2B4 is known to bind CD48 hematopoietic antigen, therefore this observation may provide the rationale why CD56dim subset expansion correlates with successful hematopoietic stem cell transplantation mediated by alloreactive NK cells against host T, DC and leukemic cells, while sparing host non-hematopoietic tissues and graft versus host disease. The assay further confirms that activation of LFA-1 on NK cells leads to their granule polarization, even if, in some cases, this also takes to an inhibition of NK cell degranulation, suggesting that LFA-1 engagement by ICAMs on target cells may differently affect NK cell response. Finally, we observed that NK cells undergo a time-dependent spontaneous (cytokine-independent) activation after blood withdrawal, an aspect that may strongly bias the evaluation of the resting NK cell response. Altogether our data may pave the way to develop new NK cell activation and expansion strategies that target the highly cytotoxic CD56dim NK cells and can be feasible and useful for cancer and viral infection treatment.
Highlights
Natural killer (NK) cells are large granular cytotoxic lymphocytes considered part of the innate immune system
NK cell degranulation induced by anti-NKp46 monoclonal antibodies (mAbs) in combination with mAbs to CD2, DNAM-1 and 2B4 coactivating receptors was first analysed in peripheral blood resting NK cells
Ex-vivo activated NK cells can be exploited to counter cancer cells after their injection; we have only limited knowledge regarding the activating and inhibitory signals induced in the different NK cell subsets
Summary
Natural killer (NK) cells are large granular cytotoxic lymphocytes considered part of the innate immune system. They provide rapid responses against virally infected and tumour cells; for these features, NK cells have been successfully employed in several immunotherapeutic strategies [1,2,3,4,5,6]. Main actors of this mechanism are HLA class I (HLA-I)-specific inhibitory receptors, killer cell immunoglobulin–like receptors (KIRs) and C-type lectin (CD94-NKG2A), and several NK cell activating receptors [7,8,9]. MHC class I-specific inhibitory receptors allow NK cells to sense down modulations in HLA-I expression, and their own “license”
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