Glucocorticoid regulates mesenchymal cell differentiation required for perinatal lung morphogenesis and function

被引:22
作者
Bridges, James P. [1 ,3 ]
Sudha, Parvathi [1 ]
Lipps, Dakota [2 ]
Wagner, Andrew [2 ]
Guo, Minzhe [1 ]
Du, Yina [1 ]
Brown, Kari [1 ]
Filuta, Alyssa [1 ]
Kitzmiller, Joseph [1 ]
Stockman, Courtney [1 ]
Chen, Xiaoting [5 ]
Weirauch, Matthew T. [3 ,4 ,5 ,6 ]
Jobe, Alan H. [1 ,3 ]
Whitsett, Jeffrey A. [1 ,3 ]
Xu, Yan [1 ,3 ,4 ]
机构
[1] Cincinnati Childrens Hosp Med Ctr, Sect Pulm Biol, Perinatal Inst, Cincinnati, OH 45229 USA
[2] Univ Cincinnati, Coll Engn & Appl Sci, Cincinnati, OH USA
[3] Univ Cincinnati, Sch Med, Dept Pediat, Cincinnati, OH 45221 USA
[4] Cincinnati Childrens Hosp Med Ctr, Div Biomed Informat, Cincinnati, OH 45229 USA
[5] Cincinnati Childrens Hosp Med Ctr, Ctr Autoimmune Genom & Etiol, Cincinnati, OH 45229 USA
[6] Cincinnati Childrens Hosp Med Ctr, Div Dev Biol, Cincinnati, OH 45229 USA
关键词
glucocorticoid signaling; matrix fibroblast; regulatory network systems biology; single cell; TRANSCRIPTION FACTOR; GENE-EXPRESSION; BETA-CATENIN; FETAL LUNG; STEM-CELLS; PROTEIN-A; RECEPTOR; CHROMATIN; BETA-1-INTEGRIN; IDENTIFICATION;
D O I
10.1152/ajplung.00459.2019
中图分类号
Q4 [生理学];
学科分类号
071003 ;
摘要
While antenatal glucocorticoids are widely used to enhance lung function in preterm infants, cellular and molecular mechanisms by which glucocorticoid receptor (GR) signaling influences lung maturation remain poorly understood. Deletion of the glucocorticoid receptor gene (Nr3c1) from fetal pulmonary mesenchymal cells phenocopied defects caused by global Nr3c1 deletion, while lung epithelial- or endothelial-specific Nr3c1 deletion did not impair lung function at birth. We integrated genome-wide gene expression profiling, ATAC-seq, and single cell RNA-seq data in mice in which GR was deleted or activated to identify the cellular and molecular mechanisms by which glucocorticoids control prenatal lung maturation. GR enhanced differentiation of a newly defined proliferative mesenchymal progenitor cell (PMP) into matrix fibroblasts (MFBs), in part by directly activating extracellular matrix-associated target genes, including Fn1, Col16a4, and Eln and by modulating VEGF, JAK-STAT, and WNT signaling. Loss of mesenchymal GR signaling blocked fibroblast progenitor differentiation into mature MFBs, which in turn increased proliferation of SOX9+ alveolar epithelial progenitor cells and inhibited differentiation of mature alveolar type II (AT(2)) and ATI cells. GR signaling controls genes required for differentiation of a subset of proliferative mesenchymal progenitors into matrix fibroblasts, in turn, regulating signals controlling AT(2)/AT(1) progenitor cell proliferation and differentiation and identifying cells and processes by which glucocorticoid signaling regulates fetal lung maturation.
引用
收藏
页码:L239 / L255
页数:17
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