BTK inhibitor–induced defects in human neutrophil effector activity against Aspergillus fumigatus are restored by TNF-α
Diego A. Vargas-Blanco, Olivia W. Hepworth, Kyle J. Basham, Patricia Simaku, Arianne J. Crossen, Kyle D. Timmer, Alex Hopke, Hannah Brown Harding, Steven R. Vandal, Kirstine N. Jensen, Daniel J. Floyd, Jennifer L. Reedy, Christopher Reardon, Michael K. Mansour, Rebecca A. Ward, Daniel Irimia, Jeremy S. Abramson, Jatin M. Vyas
Diego A. Vargas-Blanco, Olivia W. Hepworth, Kyle J. Basham, Patricia Simaku, Arianne J. Crossen, Kyle D. Timmer, Alex Hopke, Hannah Brown Harding, Steven R. Vandal, Kirstine N. Jensen, Daniel J. Floyd, Jennifer L. Reedy, Christopher Reardon, Michael K. Mansour, Rebecca A. Ward, Daniel Irimia, Jeremy S. Abramson, Jatin M. Vyas
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Research Article Immunology Infectious disease

BTK inhibitor–induced defects in human neutrophil effector activity against Aspergillus fumigatus are restored by TNF-α

Abstract

Inhibition of Bruton’s tyrosine kinase (BTK) through covalent modifications of its active site (e.g., ibrutinib [IBT]) is a preferred treatment for multiple B cell malignancies. However, IBT-treated patients are more susceptible to invasive fungal infections, although the mechanism is poorly understood. Neutrophils are the primary line of defense against these infections; therefore, we examined the effect of IBT on primary human neutrophil effector activity against Aspergillus fumigatus. IBT significantly impaired the ability of neutrophils to kill A. fumigatus and potently inhibited reactive oxygen species (ROS) production, chemotaxis, and phagocytosis. Importantly, exogenous TNF-α fully compensated for defects imposed by IBT and newer-generation BTK inhibitors and restored the ability of neutrophils to contain A. fumigatus hyphal growth. Blocking TNF-α did not affect ROS production in healthy neutrophils but prevented exogenous TNF-α from rescuing the phenotype of IBT-treated neutrophils. The restorative capacity of TNF-α was independent of transcription. Moreover, the addition of TNF-α immediately rescued ROS production in IBT-treated neutrophils, indicating that TNF-α worked through a BTK-independent signaling pathway. Finally, TNF-α restored effector activity of primary neutrophils from patients on IBT therapy. Altogether, our data indicate that TNF-α rescued the antifungal immunity block imposed by inhibition of BTK in primary human neutrophils.

Authors

Diego A. Vargas-Blanco, Olivia W. Hepworth, Kyle J. Basham, Patricia Simaku, Arianne J. Crossen, Kyle D. Timmer, Alex Hopke, Hannah Brown Harding, Steven R. Vandal, Kirstine N. Jensen, Daniel J. Floyd, Jennifer L. Reedy, Christopher Reardon, Michael K. Mansour, Rebecca A. Ward, Daniel Irimia, Jeremy S. Abramson, Jatin M. Vyas

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Figure 3

TNF-α rescued IBT-induced immune defects in neutrophils against A. fumigatus.

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TNF-α rescued IBT-induced immune defects in neutrophils against A. fumig...
Human neutrophils were treated with 0.03 μM IBT, 0.3 μM IBT, or DMSO for 30 min followed by a 4h incubation with TNF-α and coincubated with A. fumigatus B5233 strain for all figure panels. For all panels, data are representative of at least 3 independent experiments. (A) Neutrophils were incubated with A. fumigatus (MOI:0.25) for 5h, and metabolic activity was measured by resazurin assay. Data calculated through time course study (see raw data in the Supporting Data Values file) and panel represent the output from linear regression analysis using Gompertz fit with percentages of growth inhibition of A. fumigatus by neutrophils in reference to IBT-treated neutrophils. Data are shown as 95% CI, n = 3. Ordinary 1-way ANOVA and Tukey’s multiple-comparison test with a single pooled variance demonstrated a P < 0.001 for all TNF-α treatments versus IBT alone. (B) Neutrophils were stimulated with 1 mg/mL A. fumigatus heat-killed hyphae. ROS production was measured by chemiluminescence using lucigenin. Data are shown as mean ± SD, n = 3. (C) Microscopy panels showing neutrophils swarm formations 200 min after coincubation. (D) Area of neutrophil swarm after 200 min. (E) Area of fungal growth normalized to the growth of A. fumigatus without neutrophils after 16h. Data are shown as mean ± SD, n = 24. Ordinary 1-way ANOVA and Tukey’s multiple-comparison test with a single pooled variance. **P < 0.01; ****P < 0.0001. (F) Neutrophils were coincubated with AF488-labeled A. fumigatus swollen spores (MOI: 10). The displayed percentage of phagocytic neutrophils (CD45-AF700+CD66b-APC+conidia-AF488+) was estimated based on the total number of viable neutrophils (CD45-AF700+CD66b-APC+). At minimum, 10,000 viable CD66b-APC+ events were recorded. (G) Heatmap for DEG based on log2 fold change (1.5 < log2 fold change < –1.5) and a Padj < 0.05. FDR was calculated using the Benjamini-Yekutieli method with 3 biological replicates per condition. RNA from neutrophils coincubated for 5h with A. fumigatus B5233 strain (MOI: 2.5).