Am. J. Respir. Cell Mol. Biol., Vol 16, No. 3, Mar 1997, 283-292.
Alveolar macrophages stimulated with titanium dioxide, chrysotile asbestos, and residual oil fly ash upregulate the PDGF receptor-alpha on lung fibroblasts through an IL-1beta-dependent mechanism
PM Lindroos, PG Coin, A Badgett, DL Morgan and JC Bonner
Laboratory of Pulmonary Pathobiology, National Institute of Environmental Health Sciences, Research Triangle Park, North Carolina, USA.
Enhanced proliferation of fibroblasts is a primary characteristic of lung
fibrosis. Macrophage-secreted platelet-derived growth factor (PDGF) is a
potent mitogen and chemoattractant for lung fibroblasts. The magnitude of
the fibroblast PDGF response is dependent on the number of PDGF receptor
alpha (PDGF-R alpha) relative to PDGF-R beta at the cell surface. We
recently reported that upregulation of the PDGF-R alpha subtype by
interleukin (IL)-1beta results in enhanced lung fibroblast proliferation in
response to PDGF-AA, PDGF-AB, and PDGF-BB whereas transforming growth
factor (TGF)-beta1 has the opposite effect. Both IL-1beta and TGF-beta1 are
produced by particle-activated macrophages in vivo and in vitro. We studied
the net effect of macrophage conditioned medium (MOCM), which contains both
IL-1beta and TGF-beta1, on the expression of the lung fibroblast PDGF
receptor system. MOCM obtained from unstimulated, titanium dioxide (TiO2)-,
chrysotile asbestos-, or residual oil fly ash (ROFA)-exposed macrophages in
vitro increased [125I]PDGF-AA binding 3-, 6-, 6-, and 20- fold,
respectively. These increases correlated with increased PDGF-R alpha mRNA
and protein expression as shown by northern and western assays. PDGF-AB and
-BB-stimulated [3H]thymidine incorporation by fibroblasts was enhanced 5-,
5-, 10-, and 20-fold by pretreatment with MOCM from unstimulated, TiO2-,
asbestos-, and ROFA-exposed macrophages, respectively. [125I]PDGF-AA
binding experiments using the IL-1 receptor antagonist blocked the
upregulatory effect of all MOCM samples. Latent TGF-beta1 present in MOCM
was activated by acid treatment, inhibiting upregulation by approximately
60%, a result similar to experiments with IL-1beta and TGF-beta1 mixtures.
Treatment with a TGF-beta neutralizing antibody restored full upregulatory
activity to acidified MOCM. Thus activated macrophages increase lung
fibroblast PDGF-R alpha primarily due to the secretion of IL-1beta.
Intratracheal instillation of ROFA particles in rats induced a 2-fold
increase in total lung PDGF-R alpha mRNA in vivo. These findings support
the idea that macrophage-derived IL-1beta plays a key role in the
initiation of a fibrotic response by increasing fibroblast PDGF-R alpha
expression, thereby dramatically potentiating the mitogenic response to
PDGF.
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Copyright © 1997 American Thoracic Society.
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