Am. J. Respir. Cell Mol. Biol., Vol 17, No. 1, 07 1997, 25-35.
Exogenous and endogenous transforming growth factors-beta influence elastin gene expression in cultured lung fibroblasts
SE McGowan, SK Jackson, PJ Olson, T Parekh and LI Gold
Department of Veterans Affairs Research Service, Washington, District of Columbia, USA.
Elastin, an important structural protein of the extracellular matrix,
confers elastic properties on the pulmonary alveolar interstitium. In the
alveolar wall, elastin is primarily produced postnatally by fibroblasts.
The mechanisms that regulate lung fibroblast (LF) elastin gene expression
have not been completely defined, although both transcriptional and
posttranscriptional mechanisms appear to be involved. Transforming growth
factors-beta (TGF-beta s) have been shown to increase elastin production by
cultured neonatal rat LF. Analyses of elastin gene transcription and mRNA
stability indicate that exogenous TGF-beta 1 increases the half-life of
tropoelastin mRNA by 1.5-fold and does not alter elastin gene
transcription. Interference with the functions of endogenous TGF-beta 1 in
cultured LF, through the addition of neutralizing antibodies or antisense
oligodeoxynucleotides, decreases tropoelastin and tropoelastin mRNA
production by these cells. The content of total (latent plus active)
TGF-beta s was approximately 4.5-fold greater in lungs obtained from rats
on postnatal day 8 than in lungs obtained from adults. These findings
indicate that endogenous TGF- beta s, in cultured LF, regulate elastin gene
expression, most likely by a posttranscriptional mechanism. Since others
have shown that elastin mRNA appears to have a longer half-life in neonatal
than in adult rat lungs, we hypothesize that the higher content of TGF-beta
s could contribute to the greater elastin mRNA stability in neonatal lungs.
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Copyright © 1997 American Thoracic Society.
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