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胃泌素释放肽受体基因在发育中的肺中的表达。

Expression of gastrin-releasing peptide receptor gene in developing lung.

作者信息

Wang D, Yeger H, Cutz E

机构信息

Department of Pathology, Hospital for Sick Children, Toronto, Ontario, Canada.

出版信息

Am J Respir Cell Mol Biol. 1996 May;14(5):409-16. doi: 10.1165/ajrcmb.14.5.8624245.

DOI:10.1165/ajrcmb.14.5.8624245
PMID:8624245
Abstract

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.

摘要

蛙皮素(BN)或其哺乳动物对应物胃泌素释放肽(GRP)由肺神经内分泌细胞(PNEC)产生。GRP作为一种生长因子的功能涉及肺形态发生,但其确切机制和靶细胞尚未明确。我们对胎儿和新生儿的人肺及兔肺样本进行了GRP受体(GRP-R)及其配体GRP的非放射性原位杂交(NISH)和Northern印迹分析。对于BN/GRP和增殖的肺细胞群体的免疫定位,我们分别使用了抗BN/GRP或MIB-1抗体。NISH和Northern印迹显示,GRP-R mRNA在胎兔肺妊娠第24天时表达达到峰值。在细胞水平上,GRP-R mRNA主要定位于远端气道上皮管和周围间充质,而近端气道信号减弱。与呈阴性的PNEC相比,表达GRP-R的上皮细胞对增殖抗原呈阳性标记。在人产后肺中,GRP-R mRNA的强信号定位于气道上皮细胞和黏膜下腺。兔肺和人肺中的PNEC均表达GRP的mRNA,但只有人肺中的PNEC对该肽具有免疫反应性。然而,在兔胎儿肺培养物中检测到了BN/GRP免疫反应性细胞。GRP-R在哺乳动物肺中的表达受发育调控,在气道快速生长和分化阶段在空间和时间上均达到峰值。上皮和间充质成分均表达GRP-R,这与肺形态发生过程中GRP活性的旁分泌机制一致。

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