Fibrin(ogen) exacerbates inflammatory joint disease through a mechanism linked to the integrin αMβ2 binding motif
Matthew J. Flick, … , Sherry Thornton, Jay L. Degen
Matthew J. Flick, … , Sherry Thornton, Jay L. Degen
Published October 11, 2007
Citation Information: J Clin Invest. 2007;117(11):3224-3235. https://doi.org/10.1172/JCI30134.
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Research Article Inflammation

Fibrin(ogen) exacerbates inflammatory joint disease through a mechanism linked to the integrin αMβ2 binding motif

Abstract

Fibrin deposition within joints is a prominent feature of arthritis, but the precise contribution of fibrin(ogen) to inflammatory events that cause debilitating joint damage remains unknown. To determine the importance of fibrin(ogen) in arthritis, gene-targeted mice either deficient in fibrinogen (Fib–) or expressing mutant forms of fibrinogen, lacking the leukocyte receptor integrin αMβ2 binding motif (Fibγ390–396A) or the αIIbβ3 platelet integrin-binding motif (FibγΔ5), were challenged with collagen-induced arthritis (CIA). Fib– mice exhibited fewer affected joints and reduced disease severity relative to controls. Similarly, diminished arthritis was observed in Fibγ390–396A mice, which retain full clotting function. In contrast, arthritis in FibγΔ5 mice was indistinguishable from that of controls. Fibrin(ogen) was not essential for leukocyte trafficking to joints, but appeared to be involved in leukocyte activation events. Fib– and Fibγ390–396A mice with CIA displayed reduced local expression of TNF-α, IL-1β, and IL-6, which suggests that αMβ2-mediated leukocyte engagement of fibrin is mechanistically upstream of the production of proinflammatory mediators. Supporting this hypothesis, arthritic disease driven by exuberant TNF-α expression was not impeded by fibrinogen deficiency. Thus, fibrin(ogen) is an important, but context-dependent, determinant of arthritis, and one mechanism linking fibrin(ogen) to joint disease is coupled to αMβ2-mediated inflammatory processes.

Authors

Matthew J. Flick, Christine M. LaJeunesse, Kathryn E. Talmage, David P. Witte, Joseph S. Palumbo, Malinda D. Pinkerton, Sherry Thornton, Jay L. Degen

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Figure 6

Fibrinogen deficiency does not alter anti-CII antibody production, T cell reactivity, or neutrophil accumulation in joints of mice with CIA.

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Fibrinogen deficiency does not alter anti-CII antibody production, T cel...
(A) Determination of anti-CII specific IgG antibody titers by ELISA using plasma harvested at day 40 of the CIA protocol from Fib+ and Fib mice (n = 12 per group). Titers are expressed as arbitrary units relative to titers found in wild-type DBA/1 mice at day 28 of CIA. Results are expressed as mean ± SEM. (B) Cellular response to CII. Spleen cells were harvested from Fib+ and Fib mice (n = 3 per group) at day 40 of the CIA protocol and stimulated with 30 μg/ml CII or anti-CD3 activating T cell receptor antibody. Results are mean ± SEM of [3H]TdR incorporated in cpm. (C) Determination of neutrophil-derived MPO activity in total protein extracts from hind paws of Fib+ and Fib mice that were unchallenged (n = 4 per genotype), at day 28 of CIA (n = 8 per genotype), and at day 40 of CIA (n = 16 per genotype). Results are mean ± SEM. *P < 0.03, Student’s t test.