Antibody treatment ameliorates inflammation in experimental arthritis.

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Antibody treatment ameliorates inflammation in experimental arthritis. Antibody treatment ameliorates inflammation in experimental arthritis. (A and B) Synovial biopsies from the Birmingham early arthritis cohort were stained with anti-FBG antibodies. Quantification of the number of positive pixels per microgram biopsy was performed in tissue from people with early RA (undiagnosed synovitis of less than 3 months, patients who go on to be diagnosed with RA), people with synovial inflammation that spontaneously resolved (undiagnosed synovitis of less than 3 months that disappears by itself) (resolving) and people with established RA (diagnosed disease, greater than 3 months’ duration) (A). Anti-FBG staining was observed in areas of fibrosis in inflamed synovia (left panel: red anti-FBG, green anti-CD90, blue antipodoplanin) and around areas of vascularisation underneath endothelial cells (centre panel: red anti-FBG, green anti-CD31). No staining was observed with isotype controls in place of primary antibodies (right panel). Scale bars 50 µm (B). (C) Mixed populations of cells isolated from RA synovial membranes were stimulated with 1 µM recombinant human tenascin-C FBG or 1 ng/mL LPS, which had been preincubated with either C3 or isotype control antibody. After 24 hours, supernatants were taken and cytokine ELISAs were performed. Data are shown as the mean±SEM from three independent donors. One-way analysis of variance (ANOVA) was performed to determine significance of C3 inhibition compared with isotype control. *p=0.02, ***p<0.0001. (D–F) Rats were injected with bovine type II collagen intradermally on day 0 and day 7. Treatments of PBS (vehicle control) and C3 at 1, 3 or 10 mg/kg were administered twice weekly throughout the experiment by intravenous injection (10 animals per treatment group). Animals were scored for clinical signs of disease three times per week, and the mean±SEM is shown (D). Paw volumes were measured using a plethysmometer on days 0, 14, 21 and 28, and the mean change±SEM normalised to the day 0 measurements is shown (E). Two-way was carried out to test for significance of changes between vehicle and treatment groups. ****p<0.0001, ***p<0.001, **p<0.01, *p<0.05. (F) At termination on day 28, hind limbs were assessed for histological signs of inflammation, articular cartilage damage and damage to the underlying metaphyseal bone. A χ2 test for trend was used to confirm that the presence or absence of histopathological signs is associated with antibody treatment (χ2=9.098, p=0.003), with only 3 of 20 paws were free of any sign of histopathology in the vehicle treated group, whereas 11 of 20 paws were disease free in the 10 mg/kg treated group (table). Representative histological images of destructive arthritis (vehicle treated) and a normal joint (10 mg/kg) are shown (right panels). FBG, fibrinogen-like globe; IL, interleukin; RA, rheumatoid arthritis; TNF, tumour necrosis factor. Susan R Aungier et al. Ann Rheum Dis 2019;78:186-191 ©2019 by BMJ Publishing Group Ltd and European League Against Rheumatism