Am. J. Respir. Cell Mol. Biol., Vol 14, No. 5, May 1996, 409-416.
Expression of gastrin-releasing peptide receptor gene in developing lung
D Wang, H Yeger and E Cutz
Department of Pathology, Hospital for Sick Children, Toronto, Ontario, Canada.
Bombesin (BN) or its mammalian counterpart, Gastrin-releasing peptide (GRP)
is produced by pulmonary neuroendocrine cells (PNEC). The function of GRP
as a growth factor involves lung morphogenesis, but the precise mechanism
and the target cells have not been defined. We used a nonradioactive in
situ hybridization (NISH) and Northern blot analysis for both GRP receptor
(GRP-R) and its ligand GRP on samples of fetal and newborn human and rabbit
lung. For immunolocalization of BN/GRP and the proliferating lung cell
population we used anti-BN/GRP or MIB-1 antibodies, respectively. NISH and
Northern blot showed peak expression of GRP-R mRNA on day 24 gestation in
the fetal rabbit lung. At the cellular level, GRP-R mRNA was localized
mainly in the distal airway epithelial tubes and surrounding mesenchyme,
whereas proximal airways showed decreased signal. Epithelium expressing
GRP-R showed positive labeling for proliferation antigen in contrast to
PNEC, which were negative. In human post-natal lung, strong signal for
GRP-R mRNA was localized in the airway epithelial cells and submucosal
glands. PNEC in both rabbit and human lung expressed mRNA for GRP, but only
in human lung were they immunoreactive for the peptide. However BN/GRP
immunoreactive cells were detected in rabbit fetal lung culture. The
expression of GRP-R in mammalian lung is developmentally regulated, peaking
both spatially and temporally during the phase of rapid airway growth and
differentiation. Both epithelial and mesenchymal components express GRP-R
consistent with paracrine mechanism for GRP activity during lung
morphogenesis.
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Copyright © 1996 American Thoracic Society.
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