Oncostatin M acting via OSMR, augments the actions of IL-1 and TNF in synovial fibroblasts

Le Goff, B.; Singbrant, Sofie; Tonkin, B. A.; Martin, T. J.; Romas, E.; Sims, N. A.; Walsh, N. C.

Oncostatin M acting via OSMR, augments the actions of IL-1 and TNF in synovial fibroblasts

Mark

Le Goff, B. ; Singbrant, Sofie ^LU ; Tonkin, B. A. ; Martin, T. J. ; Romas, E. ; Sims, N. A. and Walsh, N. C. (2014) In Cytokine 68(2). p.9-101

Abstract: OBJECTIVE: To identify how the gp130-signaling cytokine oncostatin M (OSM), acting alone or in concert with IL-1beta or TNFalpha, affects synovial fibroblast expression of genes relevant to inflammation and bone erosion in inflammatory arthritis. METHODS: Synovial fibroblasts (SFs) were isolated from non-arthritic wild type (WT) or OSM receptor deficient (OSMR(-/-)) mice and stimulated with OSM, IL-1beta or TNFalpha and their combinations. Cytokine gene expression was assessed by quantitative RT-PCR. ELISA, flow cytometry and immunohistochemistry identified protein expression. Gene expression patterns were confirmed in SFs isolated from patients with osteoarthritis (OASFs) and rheumatoid arthritis (RASFs). RESULTS: Expression of OSM and... (More); OBJECTIVE: To identify how the gp130-signaling cytokine oncostatin M (OSM), acting alone or in concert with IL-1beta or TNFalpha, affects synovial fibroblast expression of genes relevant to inflammation and bone erosion in inflammatory arthritis. METHODS: Synovial fibroblasts (SFs) were isolated from non-arthritic wild type (WT) or OSM receptor deficient (OSMR(-/-)) mice and stimulated with OSM, IL-1beta or TNFalpha and their combinations. Cytokine gene expression was assessed by quantitative RT-PCR. ELISA, flow cytometry and immunohistochemistry identified protein expression. Gene expression patterns were confirmed in SFs isolated from patients with osteoarthritis (OASFs) and rheumatoid arthritis (RASFs). RESULTS: Expression of OSM and its receptors, gp130, OSMR and LIFR, was increased in synovial tissue from the mouse antigen-induced arthritis model. In isolated WT mouse synovial fibroblasts OSM alone, or in synergy with IL-1beta, or together with TNFalpha, potently induced expression of the pro-inflammatory cytokine IL-6. OSM also induced a sustained increase in mRNA levels of the pro-osteoclastic cytokine RANKL. Combining OSM with IL-1beta, but not with TNFalpha, further increased RANKL expression. Importantly these effects of OSM were all dependent on the expression of OSMR. Furthermore, OSM also increased expression of its own receptors, gp130 and OSMR and the IL-1 receptor, IL1-R1; the latter effects were also observed in both human OASFs and RASFs. CONCLUSION: Together our data suggests that OSM signaling via OSMR in SFs has the potential to contribute significantly to joint destruction in inflammatory arthritis. It not only induces expression of pro-inflammatory and pro-osteoclastic cytokines but can also augment its own actions and that of IL-1 by inducing expression of OSMR and IL-1R1. (Less)

Please use this url to cite or link to this publication: https://lup.lub.lu.se/record/8594803

author

Le Goff, B. ; Singbrant, Sofie ^LU ; Tonkin, B. A. ; Martin, T. J. ; Romas, E. ; Sims, N. A. and Walsh, N. C.

organization

StemTherapy: National Initiative on Stem Cells for Regenerative Therapy

publishing date

2014

type

Contribution to journal

publication status

published

subject

Rheumatology and Autoimmunity

keywords

Synovial Membrane/*pathology, Rheumatoid/genetics/pathology, Animals, Humans, Tumor Necrosis Factor-alpha/*metabolism, Arthritis, Il-1, Il-6, Oncostatin M, Synovial fibroblast, Interleukin-1beta/genetics/*metabolism, Receptors, Oncostatin M/deficiency/*metabolism, Inbred C57BL, Gene Expression Regulation, Mice, Oncostatin M/*metabolism, Fibroblasts/*metabolism, Osteoprotegerin/genetics/metabolism, RNA, Messenger/genetics/metabolism, RANK Ligand/genetics/metabolism, Interleukin-1/metabolism

in

Cytokine

volume

68

issue

2

pages

9 - 101

publisher

Academic Press

external identifiers

scopus:84900821938

ISSN

1096-0023

DOI

10.1016/j.cyto.2014.04.001

language

English

LU publication?

no

additional info

2

id

1215cb9e-0e7a-46f1-a42b-f1b8a12b9f0b (old id 8594803)

date added to LUP

2016-04-01 13:15:18

date last changed

2022-01-27 18:07:47

@article{1215cb9e-0e7a-46f1-a42b-f1b8a12b9f0b,
  abstract     = {{OBJECTIVE: To identify how the gp130-signaling cytokine oncostatin M (OSM), acting alone or in concert with IL-1beta or TNFalpha, affects synovial fibroblast expression of genes relevant to inflammation and bone erosion in inflammatory arthritis. METHODS: Synovial fibroblasts (SFs) were isolated from non-arthritic wild type (WT) or OSM receptor deficient (OSMR(-/-)) mice and stimulated with OSM, IL-1beta or TNFalpha and their combinations. Cytokine gene expression was assessed by quantitative RT-PCR. ELISA, flow cytometry and immunohistochemistry identified protein expression. Gene expression patterns were confirmed in SFs isolated from patients with osteoarthritis (OASFs) and rheumatoid arthritis (RASFs). RESULTS: Expression of OSM and its receptors, gp130, OSMR and LIFR, was increased in synovial tissue from the mouse antigen-induced arthritis model. In isolated WT mouse synovial fibroblasts OSM alone, or in synergy with IL-1beta, or together with TNFalpha, potently induced expression of the pro-inflammatory cytokine IL-6. OSM also induced a sustained increase in mRNA levels of the pro-osteoclastic cytokine RANKL. Combining OSM with IL-1beta, but not with TNFalpha, further increased RANKL expression. Importantly these effects of OSM were all dependent on the expression of OSMR. Furthermore, OSM also increased expression of its own receptors, gp130 and OSMR and the IL-1 receptor, IL1-R1; the latter effects were also observed in both human OASFs and RASFs. CONCLUSION: Together our data suggests that OSM signaling via OSMR in SFs has the potential to contribute significantly to joint destruction in inflammatory arthritis. It not only induces expression of pro-inflammatory and pro-osteoclastic cytokines but can also augment its own actions and that of IL-1 by inducing expression of OSMR and IL-1R1.}},
  author       = {{Le Goff, B. and Singbrant, Sofie and Tonkin, B. A. and Martin, T. J. and Romas, E. and Sims, N. A. and Walsh, N. C.}},
  issn         = {{1096-0023}},
  keywords     = {{Synovial Membrane/*pathology; Rheumatoid/genetics/pathology; Animals; Humans; Tumor Necrosis Factor-alpha/*metabolism; Arthritis; Il-1; Il-6; Oncostatin M; Synovial fibroblast; Interleukin-1beta/genetics/*metabolism; Receptors; Oncostatin M/deficiency/*metabolism; Inbred C57BL; Gene Expression Regulation; Mice; Oncostatin M/*metabolism; Fibroblasts/*metabolism; Osteoprotegerin/genetics/metabolism; RNA; Messenger/genetics/metabolism; RANK Ligand/genetics/metabolism; Interleukin-1/metabolism}},
  language     = {{eng}},
  number       = {{2}},
  pages        = {{9--101}},
  publisher    = {{Academic Press}},
  series       = {{Cytokine}},
  title        = {{Oncostatin M acting via OSMR, augments the actions of IL-1 and TNF in synovial fibroblasts}},
  url          = {{http://dx.doi.org/10.1016/j.cyto.2014.04.001}},
  doi          = {{10.1016/j.cyto.2014.04.001}},
  volume       = {{68}},
  year         = {{2014}},
}

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Oncostatin M acting via OSMR, augments the actions of IL-1 and TNF in synovial fibroblasts