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Regulation of fibroblast lipid storage and myofibroblast phenotypes during alveolar septation in mice

机译:小鼠肺泡分离过程中成纤维细胞脂质存储和成肌纤维细胞表型的调节

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摘要

Signaling through platelet-derived growth factor receptor-α (PDGFRα) is required for alveolar septation and participates in alveolar regeneration after pneumonectomy. In both adipose tissue and skeletal muscle, bipotent pdgfrα-expressing progenitors expressing delta-like ligand-1 or sex-determining region Y box 9 (Sox9) may differentiate into either lipid storage cells or myofibroblasts. We analyzed markers of mesenchymal progenitors and differentiation in lung fibroblasts (LF) with different levels (absent, low, or high) of pdgfrα gene expression. A larger proportion of pdgfrα-expressing than nonexpressing LF contained Sox9. Neutral lipids, CD166, and Tcf21 were more abundant in LF with a lower compared with a higher level of pdgfrα gene expression. PDGF-A increased Sox9 in primary LF cultures, suggesting that active signaling through PDGFRα is required to maintain Sox9. As alveolar septation progresses from postnatal day (P) 8 to P12, fewer pdgfrα-expressing LF contain Sox9, whereas more of these LF contain myocardin-like transcription factor-A, showing that Sox9 diminishes as LF become myofibroblasts. At P8, neutral lipid droplets predominate in LF with the lower level of pdgfrα gene expression, whereas transgelin (tagln) was predominantly expressed in LF with higher pdgfrα gene expression. Targeted deletion of pdgfrα in LF, which expressed tagln, reduced Sox9 in α-actin (α-SMA, ACTA2)-containing LF, whereas it increased the abundance of cell surface delta-like protein-1 (as well as peroxisome proliferator-activated receptor-γ and tcf21 mRNA in LF, which also expressed stem cell antigen-1). Thus pdgfrα deletion differentially alters delta-like protein-1 and Sox9, suggesting that targeting different downstream pathways in PDGF-A-responsive LF could identify strategies that promote lung regeneration without initiating fibrosis.
机译:肺泡分隔需要通过血小板衍生的生长因子受体-α(PDGFRα)进行信号传导,并参与肺切除术后的肺泡再生。在脂肪组织和骨骼肌中,表达δ样配体-1或性别决定区域Y框9(Sox9)的表达双能pdgfrα的祖细胞可能分化为脂质存储细胞或成肌纤维细胞。我们分析了pdgfrα基因表达水平不同(不存在,低或高)的肺成纤维细胞(LF)中的间充质祖细胞和分化标记。表达pdgfrα的比例比不表达LF的比例更大,其中包含Sox9。 LF中的中性脂质CD166和Tcf21含量较高,而pdgfrα基因表达水平较高。 PDGF-A在原代LF培养物中增加了Sox9,这表明维持PDx-α需要通过PDGFRα的主动信号传导。随着肺泡分隔从出生后第8天发展到P12,表达pdgfrα的LF中包含Sox9的较少,而这些LF中包含心肌样转录因子-A的更多,这表明随着LF成为成肌纤维细胞,Sox9逐渐减少。在P8,中性脂质滴在LF中以较低的pdgfrα基因表达水平占主导地位,而转胶蛋白(tagln)在LF中以较高的pdgfrα基因表达水平主要表达。 LF中有针对性的pdgfrα缺失表达tagln,减少了含α-肌动蛋白(α-SMA,ACTA2)的LF中的Sox9,而它却增加了细胞表面δ样蛋白1(以及过氧化物酶体增殖物激活的)的丰度LF中的受体-γ和tcf21 mRNA,也表达干细胞抗原-1)。因此,pdgfrα缺失差异性地改变了delta-like蛋白1和Sox9,这表明在PDGF-A响应性LF中靶向不同的下游途径可以确定促进肺再生而不启动纤维化的策略。

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