Exploring the association between circulating endothelial protein C receptor and disease activity of rheumatoid arthritis in a pilot study

Author:

Xue Meilang12ORCID,Lin Haiyan12ORCID,Lynch Tom2ORCID,Bereza-Malcolm Lara12ORCID,Sinnathurai Premarani23ORCID,Thomas Ranjeny4ORCID,Keen Helen56ORCID,Hill Catherine78ORCID,Lester Susan78ORCID,Wechalekar Mihir910ORCID,March Lyn23ORCID

Affiliation:

1. Sutton Arthritis Research Laboratory, Sydney Musculoskeletal Health, Kolling Institute, Faculty of Medicine and Health, The University of Sydney , Sydney, NSW, Australia

2. The Australian Arthritis and Autoimmune Biobank Collaborative (A3BC), Sydney Musculoskeletal Health, Kolling Institute, Faculty of Medicine and Health, The University of Sydney and the Northern Sydney Local Health District , Sydney, NSW, Australia

3. Department of Rheumatology, Royal North Shore Hospital , Syndey, NSW, Australia

4. Frazer Institute, Translational Research Institute, The University of Queensland , Brisbane, QLD, Australia

5. Medical School, The University of Western Australia , Perth, WA, Australia

6. Department of Rheumatology, Fiona Stanley Hospital , Murdoch, WA, Australia

7. Adelaide Medical School, The University of Adelaide , Adelaide, SA, Australia

8. Rheumatology Research Group, Paediatrics, and Paediatric Rheumatology, Basil Hetzel Institute and The Queen Elizabeth Hospital , Adelaide, SA, Australia

9. Rheumatology Synovial Tissue Translational Research Group, Flinders University , Adelaide, SA, Australia

10. Rheumatology Unit, Flinders Medical Centre , Adelaide, SA, Australia

Abstract

Abstract Objectives To investigate whether circulating endothelial protein C receptor (EPCR) is associated with disease activity and inflammatory markers in rheumatoid arthritis. Methods Thirty-eight RA patients and 21 healthy controls (HC) were recruited via the A3BC biobank. Peripheral blood mononuclear cells and plasma were isolated from the blood of these participants. Plasma soluble (s)EPCR, IL-6, IL-17 and sCD14 were measured by enzyme-linked immunosorbent assay, cell membrane-associated (m)EPCR by flow cytometry; EPCR gene H3 single nucleotide polymorphism (SNP), which contributes to high plasma sEPCR levels, by PCR and DNA sequencing. Data were analysed using FlowJo10 and GraphPad Prism 10. Results RA patients had higher levels of mEPCR on T cells and plasma sEPCR compared with HC. No difference in the EPCR gene H3 SNP G genotype frequency was found between RA and HC. This SNP was significantly correlated with higher sEPCR levels in HC but not in RA patients. In RA, plasma sEPCR levels were positively correlated with IL-6, IL-17, sCD14, anti-CCP and rheumatoid factor. In contrast, mEPCR levels on T cells and natural killer cells (NK) were inversely associated with disease activity measures including 28/66 swollen joint count, 28/68 tender joint count and/or DAS28-CRP/ESR scores, and positively correlated with EPCR gene H3 SNP, which was also correlated with lower disease activity measures in RA. Conclusion Our findings suggest that EPCR may play an important role in RA, with plasma sEPCR being potentially associated with inflammatory markers and mEPCR and the EPCR gene H3 SNP possibly related to disease activity measures.

Funder

Lincoln Centre, the Ulysses Club, the Woodend Foundation

Department of Rheumatology, Royal North Shore Hospital

Publisher

Oxford University Press (OUP)

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