CXCL17 binds efficaciously to glycosaminoglycans with the potential to modulate chemokine signaling

Sean P Giblin; Sashini Ranawana; Shyreen Hassibi; Holly L Birchenough; Kyle T Mincham; Robert J Snelgrove; Tomoko Tsuchiya; Shiro Kanegasaki; Douglas Dyer; James E Pease

doi:10.3389/fimmu.2023.1254697

CXCL17 binds efficaciously to glycosaminoglycans with the potential to modulate chemokine signaling

Front Immunol. 2023 Oct 24:14:1254697. doi: 10.3389/fimmu.2023.1254697. eCollection 2023.

Authors

Affiliations

¹ National Heart and Lung Institute, Imperial College London, London, United Kingdom.
² Wellcome Centre for Cell-Matrix Research, Lydia Becker Institute of Immunology and Inflammation, Faculty of Biology, Medicine and Health, Manchester Academic Health Science Centre, University of Manchester, Manchester, United Kingdom.
³ Research Institute, National Center for Global Health and Medicine, Shinjuku-ku, Japan.
⁴ Heavy Ion Medical Center, Gunma University, Maebashi, Japan.
⁵ Geoffrey Jefferson Brain Research Centre, Manchester Academic Health Science Centre, Northern Care Alliance NHS Group, University of Manchester, Manchester, United Kingdom.

Abstract

Introduction: CXCL17 is a mucosally secreted protein, and the most recently identified human chemokine, an assignment based on protein fold prediction and chemotactic activity for leukocytes. However, these credentials have been the subject of much recent discussion and no experimental evidence has been presented regarding the definitive structure of CXCL17. In this study, we evaluated the structural and chemoattractant credentials of CXCL17 to better characterize this molecule, and gain deeper insights into its functional role as a glycosaminoglycan (GAG) binding protein.

Methods: In the absence of structural information, in silico modeling techniques assessed the likelihood of CXCL17 adopting a chemokine fold. Recombinant CXCL17 was synthesized in mammalian and prokaryotic systems. Modified Boyden chamber and real-time chemotaxis assays assessed the ability of CXCL17 to promote chemotaxis of murine splenocytes, human neutrophils, and CXCR1 transfectants. The efficacy of CXCL17 binding to GAGs was quantified with solid-phase assays and bio-layer interferometry techniques.

Results: All modeling efforts failed to support classification of CXCL17 as a chemokine based on its predicted conformation. Recombinant CXCL17 was observed to dimerize as a function of concentration, a characteristic of several chemokines. Contrary to a previous report, CXCL17 was not chemotactic for murine splenocytes, although it was a low-potency chemoattractant for human neutrophils at micromolar concentrations, several orders of magnitude higher than those required for CXCL8. As anticipated owing to its highly basic nature, CXCL17 bound to GAGs robustly, with key C-terminal motifs implicated in this process. While inactive via CXCR1, CXCL17 was found to inhibit CXCR1-mediated chemotaxis of transfectants to CXCL8 in a dose-dependent manner.

Discussion: In summary, despite finding little evidence for chemokine-like structure and function, CXCL17 readily bound GAGs, and could modulate chemotactic responses to another chemokine in vitro. We postulate that such modulation is a consequence of superior GAG binding, and that C-terminal fragments of CXCL17 may serve as prototypic inhibitors of chemokine function.

Keywords: CXCL8; CXCR1; chemokine; chemotaxis; glycosaminoglycan (GAG); model; mucosal; neutrophil.

Publication types

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

MeSH terms

Animals
Chemokines* / metabolism
Chemokines, CXC / metabolism
Chemotaxis
Glycosaminoglycans* / metabolism
Humans
Mammals / metabolism
Mice
Neutrophils / metabolism

Substances

Glycosaminoglycans
Chemokines
CXCL17 protein, human
Chemokines, CXC
CXCL17 protein, mouse

Abstract

Publication types

MeSH terms

Substances

Grants and funding