Manipulation of tissue factor-mediated basal PAR-2 signalling on macrophages determines sensitivity for IFNγ responsiveness and significantly modifies the phenotype of murine DTH

Hannah Wilkinson; Hugh Leonard; Michael G Robson; Richard Smith; ElLi Tam; John H McVey; Daniel Kirckhofer; Daxin Chen; Anthony Dorling

doi:10.3389/fimmu.2022.999871

Manipulation of tissue factor-mediated basal PAR-2 signalling on macrophages determines sensitivity for IFNγ responsiveness and significantly modifies the phenotype of murine DTH

Front Immunol. 2022 Sep 12:13:999871. doi: 10.3389/fimmu.2022.999871. eCollection 2022.

Authors

Hannah Wilkinson¹, Hugh Leonard¹, Michael G Robson¹, Richard Smith¹, ElLi Tam¹, John H McVey², Daniel Kirckhofer³, Daxin Chen¹, Anthony Dorling¹

Affiliations

¹ Department of Inflammation Biology, School of Immunology & Microbial Sciences, King's College London, Guy's Hospital, London, United Kingdom.
² School of Bioscience & Medicine, Faculty of Health and Medical Sciences, University of Surrey, Guildford, United Kingdom.
³ Department of Early Discovery Biochemistry, Genentech Inc., South San Francisco, CA, United States.

Abstract

Background: Tissue factor (TF) generates proteases that can signal through PAR-1 and PAR-2. We have previously demonstrated PAR-1 signalling primes innate myeloid cells to be exquisitely sensitive to interferon-gamma (IFNγ). In this work we explored how TF mediated PAR-2 signalling modulated responsiveness to IFNγ and investigated the interplay between PAR-1/-2 signalling on macrophages.

Methodology: We characterised how TF through PAR-2 influenced IFNγ sensitivity in vitro using PCR and flow cytometry. and how it influenced oxazolone-induced delayed type hypersensitivity (DTH) responses in vivo. We investigated how basal signalling through PAR-2 influenced PAR-1 signalling using a combination of TF-inhibitors and PAR-1 &-2 agonists and antagonists. Finally, we investigated whether this system could be targeted therapeutically using 3-mercaptopropionyl-F-Cha-Cha-RKPNDK (3-MP), which has actions on both PAR-1 and -2.

Results: TF delivered a basal signal through PAR-2 that upregulated SOCS3 expression and blunted M1 polarisation after IFNγ stimulation, opposing the priming achieved by signalling through PAR-1. PAR-1 and -2 agonists or antagonists could be used in combination to modify this basal signal in vitro and in vivo. 3-MP, by virtue of its PAR-2 agonist properties was superior to agents with only PAR-1 antagonist properties at reducing M1 polarisation induced by IFNγ and suppressing DTH. Tethering a myristoyl electrostatic switch almost completely abolished the DTH response.

Conclusions: TF-mediated signalling through PARs-1 and -2 act in a homeostatic way to determine how myeloid cells respond to IFNγ. 3-MP, an agent that simultaneously inhibits PAR-1 whilst delivering a PAR-2 signal, can almost completely abolish immune responses dependent on M1 polarisation, particularly if potency is enhanced by targeting to cell membranes; this has potential therapeutic potential in multiple diseases.

Keywords: innate immunity; macrophage; protease (proteinase)-activated receptor; thrombin; type IV hypersensitivity.

Publication types

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

MeSH terms

Animals
Interferon-gamma* / genetics
Macrophages
Mice
Oxazolone
Peptide Hydrolases / genetics
Phenotype
Receptor, PAR-1 / metabolism
Thromboplastin* / metabolism

Substances

Receptor, PAR-1
Oxazolone
Interferon-gamma
Thromboplastin
Peptide Hydrolases

Abstract

Publication types

MeSH terms

Substances

Grants and funding