Antagonizing FcαR1 (CD89) as treatment in IgA-mediated chronic inflammation and autoimmunity

Myrthe A M van Delft; Esil Aleyd; Richard van der Mast; Niels de Jong; Louis Boon; Peter J Simons; Marjolein van Egmond

doi:10.3389/fimmu.2023.1118539

Antagonizing FcαR1 (CD89) as treatment in IgA-mediated chronic inflammation and autoimmunity

Front Immunol. 2023 Apr 4:14:1118539. doi: 10.3389/fimmu.2023.1118539. eCollection 2023.

Authors

Myrthe A M van Delft^{1

2}, Esil Aleyd³, Richard van der Mast^{1

2}, Niels de Jong³, Louis Boon^{3

4}, Peter J Simons³, Marjolein van Egmond^{1

2

5}

Affiliations

¹ Molecular Cell Biology and Immunology, Amsterdam University Medical Center (UMC) location Vrije Universiteit Amsterdam, Amsterdam, Netherlands.
² Inflammatory Diseases, Amsterdam Institute for Infection and Immunity, Amsterdam, Netherlands.
³ Research and Development, Polpharma Biologics, Utrecht, Netherlands.
⁴ Research and Development, JJP Biologics, Warsaw, Poland.
⁵ Surgery, Amsterdam University Medical Center (UMC) Vrije Universiteit Amsterdam, Amsterdam, Netherlands.

Abstract

Introduction: Immunoglobulin A (IgA) is mostly considered as a non-inflammatory regulator at mucosal areas. However, previous work of our group showed that IgA can also be involved in disease pathology, because it provides a potent stimulus to activate neutrophils after crosslinking of surface CD89 (FcaRI), resulting in chronic inflammation and tissue damage. IgA (auto)antibodies and neutrophils are key players in various diseases, including blistering skin diseases and rheumatoid arthritis. Therefore, we generated an array of anti-CD89 monoclonal antibodies (mAbs) for therapeutic targeting of CD89. The biological activity of newly developed anti-human CD89 mAbs and their potential therapeutic capacity were investigated.

Methods: Human neutrophils were isolated from heparinized healthy donor blood. The ability of anti-CD89 mAbs to bind human neutrophils was investigated by flow cytometry. Furthermore, the capacity of these anti-CD89 mAbs to inhibit IgA-mediated phagocytosis, neutrophil extracellular trap (NET) release and migration was studied. To this end, neutrophils were pre-incubated with/without anti-CD89 mAbs after which they were stimulated with IgA-coated beads. The amount of phagocytosed beads, NET release and migrated neutrophils were subsequently analysed. In parallel, chemoattractant leukotriene B4 and lactoferrin (as a measure for degranulation) release were determined. Finally, the therapeutic potential of our prototypic anti-CD89 mAb clone 10E7 was in vivo tested in anti-mouse collagen XVII human IgA-treated transgenic CD89 mice, a preclinical model for autoimmune linear IgA bullous disease (LABD).

Results: Our results show that all generated anti-CD89 mAbs bound surface CD89 on neutrophils. Although these anti-CD89 mAbs bind to different epitopes on EC1 of CD89, they all have the capacity to inhibit IgA-mediated phagocytosis, neutrophil extracellular trap (NET) release and neutrophil migration. Moreover, IgA mediated leukotriene B4 and lactoferrin release are decreased in supernatant from anti-CD89 mAbs-treated neutrophils. Finally, anti-CD89 mAb clone 10E7, that was selected based on its selective binding profile on tissue micro arrays, reduced anti-mouse collagen XVII hIgA-induced neutrophil influx in an in vivo linear IgA bullous disease (LABD) mice model.

Conclusion: This study clearly indicates that our newly developed anti-CD89 mAbs inhibited IgA-induced neutrophil activation and reduced anti-autoantigen IgA-induced neutrophil influx in vivo, supporting further clinical development for the treatment of LABD.

Keywords: Fc alpha receptor (FcαRI); autoimmunity; chronic-inflammation (CI); immunoglobulin A; neutrophils (PMNs).

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Autoimmunity*
Immunoglobulin A*
Inflammation
Lactoferrin / metabolism
Leukotriene B4 / metabolism
Mice

Substances

Immunoglobulin A
Lactoferrin
Leukotriene B4

Grants and funding

This project was funded by Health Holland TKIPPP, project number LSHM18021, Polpharma Biologics (contributed to TKIPPP) and Netherlands Organization for Scientific Research (VICI 91814650).