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Novel APC-like properties of human NK cells directly regulate T cell activation
Jacob Hanna, … , Jane H. Buckner, Ofer Mandelboim
Jacob Hanna, … , Jane H. Buckner, Ofer Mandelboim
Published December 1, 2004
Citation Information: J Clin Invest. 2004;114(11):1612-1623. https://doi.org/10.1172/JCI22787.
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Article Immunology

Novel APC-like properties of human NK cells directly regulate T cell activation

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Abstract

Initiation of the adaptive immune response is dependent on the priming of naive T cells by APCs. Proteomic analysis of unactivated and activated human NK cell membrane–enriched fractions demonstrated that activated NK cells can efficiently stimulate T cells, since they upregulate MHC class II molecules and multiple ligands for TCR costimulatory molecules. Furthermore, by manipulating antigen administration, we show that NK cells possess multiple independent unique pathways for antigen uptake. These results highlight NK cell–mediated cytotoxicity and specific ligand recognition by cell surface–activating receptors on NK cells as unique mechanisms for antigen capturing and presentation. In addition, we analyzed the T cell–activating potential of human NK cells derived from different clinical conditions, such as inflamed tonsils and noninfected and CMV-infected uterine decidual samples, and from transporter-associated processing antigen 2–deficient patients. This in vivo analysis revealed that proinflammatory, but not immune-suppressive, microenvironmental requirements can selectively dictate upregulation of T cell–activating molecules on NK cells. Taken together, these observations offer new and unexpected insights into the direct interactions between NK and T cells and suggest novel APC-like activating functions for human NK cells.

Authors

Jacob Hanna, Tsufit Gonen-Gross, Jonathan Fitchett, Tony Rowe, Mark Daniels, Tal I. Arnon, Roi Gazit, Aviva Joseph, Karoline W. Schjetne, Alexander Steinle, Angel Porgador, Dror Mevorach, Debra Goldman-Wohl, Simcha Yagel, Michael J. LaBarre, Jane H. Buckner, Ofer Mandelboim

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Figure 7

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NK-mediated capturing of soluble immune complexes. (A) ANK cells (1 × 10...
NK-mediated capturing of soluble immune complexes. (A) ANK cells (1 × 106) were incubated with recombinant HA or BSA proteins (0.5 μg/ml) and pooled anti-HA or control sera (1 μl per well), for 180 minutes at 37_C. The cells were subsequently stained for surface expression of CD16. MFI levels are indicated for CD16– (upper left corner) and CD16+ NK cells (upper right corner). (B) The proliferative response of 5 × 104 OFR3 clone T cells to different concentrations of HA or BSA proteins, in the presence of a fixed concentration of pooled anti-HA or control sera (1 μl per well). Irradiated ANK cells (1 × 105) were used as APCs. The cells were cultured for 48 hours and pulsed with [3H]thymidine for the last 24 hours. Values are mean ± SD for triplicate samples. Prior to harvesting, 100 μl of supernatant was taken up for ELISA measurement of IL-2 and IFN-γ. Data are representative of 3 separate experiments.

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