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*
Department of Medicine, University of Maryland School of Medicine, and
Research Service, Veterans Affairs Medical Center, Baltimore, MD, 21201
Fibrosis can be an undesired consequence of activated cellular
immune responses. The purpose of this work was to determine whether
CD40 ligation and the pro-fibrotic cytokine IL-4 interact in regulating
fibroblast proliferation and collagen production, and, if so, the
mechanisms used. This study found that the combination of IL-4
and ligation of CD40 on the fibroblast cell surface had synergistic
effects in stimulating fibroblast proliferation. In contrast, CD40
ligation negated the inhibitory effects of IFN-
on fibroblast
proliferation. Western blotting analyses of fibroblast crude lysates
revealed that a potential mechanism of the synergy between CD40
ligation and IL-4 was the phosphorylation of proteins at 130 kDa and,
to a lesser degree, at 95, 85, and 75 kDa. Immunoprecipitation-Western
blotting experiments showed that phosphorylation levels of IL-4R
,
Janus kinase 1, insulin receptor substrate 1, and insulin receptor
substrate 2, factors with molecular mass close to the observed 130 kDa
major phosphorylation band, increased in response to the combined CD40
ligation and IL-4 action. In contrast, there was no evidence that
synergy was mediated by an increased expression of IL-4R
chain,
CD40, or the autocrine profibrotic cytokines IL-6 and TGF-
. These
findings suggest that CD40-CD40 ligand contacts between fibroblasts and
cells secreting IL-4 may promote the profibrotic effects of IL-4 by
affecting signal transduction and reducing the anti-fibrotic
effects of IFN-
.
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