Constitutive activation of WASp leads to abnormal cytotoxic cells with increased granzyme B and degranulation response to target cells
Joanna S. Kritikou, … , Jordan S. Orange, Lisa S. Westerberg
Joanna S. Kritikou, … , Jordan S. Orange, Lisa S. Westerberg
Published February 23, 2021
Citation Information: JCI Insight. 2021;6(6):e140273. https://doi.org/10.1172/jci.insight.140273.
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Research Article Immunology

Constitutive activation of WASp leads to abnormal cytotoxic cells with increased granzyme B and degranulation response to target cells

Abstract

X-linked neutropenia (XLN) is caused by gain-of-function mutations in the actin regulator Wiskott-Aldrich Syndrome protein (WASp). XLN patients have reduced numbers of cytotoxic cells in peripheral blood; however, their capacity to kill tumor cells remains to be determined. Here, we examined NK and T cells from 2 patients with XLN harboring the activating WASpL270P mutation. XLN patient NK and T cells had increased granzyme B content and elevated degranulation and IFN-γ production when compared with healthy control cells. Murine WASpL272P NK and T cells formed stable synapses with YAC-1 tumor cells and anti-CD3/CD28–coated beads, respectively. WASpL272P mouse T cells had normal degranulation and cytokine response whereas WASpL272P NK cells showed an enhanced response. Imaging experiments revealed that while WASpL272P CD8+ T cells had increased accumulation of actin upon TCR activation, WASpL272P NK cells had normal actin accumulation at lytic synapses triggered through NKp46 signaling but had impaired response to lymphocyte function associated antigen-1 engagement. When compared with WT mice, WASpL272P mice showed reduced growth of B16 melanoma and increased capacity to reject MHC class I–deficient cells. Together, our data suggest that cytotoxic cells with constitutively active WASp have an increased capacity to respond to and kill tumor cells.

Authors

Joanna S. Kritikou, Mariana M.S. Oliveira, Julien Record, Mezida B. Saeed, Saket M. Nigam, Minghui He, Marton Keszei, Arnika K. Wagner, Hanna Brauner, Anton Sendel, Saikiran K. Sedimbi, Stamatina Rentouli, David P. Lane, Scott B. Snapper, Klas Kärre, Peter Vandenberghe, Jordan S. Orange, Lisa S. Westerberg

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Figure 3

Murine WASpL272P NK cells have increased degranulation and IFN-γ production and normal synapse formation.

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Murine WASpL272P NK cells have increased degranulation and IFN-γ product...
(A) Degranulation and IFN-γ production in NK cells from WASp-KO, WT, and WASpL272P mice upon cross-linking of the activating receptors NKp46 or NK1.1 with antibodies. Representative plots of the IFN-γ production and degranulation (CD107a) in NK cells with anti-NKp46 (top) and anti-NK1.1 (bottom) stimulation are shown on the left and a cumulative graph of 4 experiments on the right. CD107a+IFN-γ+ NK cells include CD107a single positive (SP), IFN-γ SP, and CD107a IFN-γ double-positive (DP) cells. Each dot represents 1 mouse. WASp-KO anti-NKp46 n = 4, WT anti-NKp46 n = 14, WASpL272P anti-NKp46 n = 12, WASp-KO anti-NK1.1 n = 7, WT anti-NK1.1 n = 14, WASpL272P anti-NK1.1 n = 14. Graph shows mean values ± SEM and significance was assessed by 2-tailed Student’s t test. The average of nonresponding and CD107a/IFN-γ–responding NK cells after NK1.1 stimulation is also shown as pie charts in each genotype. (B) Imaging flow cytometry to assess synapse formation between NK cells from WASp-KO, WT, or WASpL272P mice and SNARF-1–stained YAC-1 lymphoma cells (pink). Doublets were selected as a function of area and aspect ratio and conjugates as a function of NK1.1 and SNARF-1 intensity. All conjugates were confirmed to consist of 1 NK cell and 1 YAC-1 lymphoma cell. Actin is shown in green (LifeActGFP) and granzyme B in orange. Representative images of conjugates are shown on the left, and a representative experiment of 3 is shown on the right. The Delta Centroid value indicates the extent of polarized fluorescence toward the synapse. Each dot represents 1 conjugate. WASp-KO n = 82, WT n = 161, WASpL272P n = 203. Graph shows mean values ± SEM and significance was assessed by 1-way ANOVA. *P ≤ 0.05, ***P ≤ 0.001, ****P ≤ 0.0001.