Conditional gene inactivation reveals roles for <i>Fgf10</i> and <i>Fgfr2</i> in establishing a normal pattern of epithelial branching in the mouse lung

Abler, Lisa L.; Mansour, Suzanne L.; Sun, Xin

doi:10.1002/dvdy.22032

Cited by 146 publications

(161 citation statements)

References 49 publications

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“…5C vs. B, G vs. F, J). This phenotype is similar to that obtained by Abler et al who used a general mesenchymal driver line (Dermo1 Cre ) to perform conditional gene inactivation of Fgf10 [14]. Last but not least, our research group has previously demonstrated that the gut is a major site of Fgf10 expression and that hypomorphic Fgf10 embryos (Fgf10 LacZ/2 ) suffered from cecal atresia [4].…”

Section: Discussionsupporting

confidence: 87%

“…Tomato flox/flox reporter mice (B6;129S6-Gt(ROSA)26Sor tm9(CAGtdTomato)Hze /J) [13] were purchased from Jackson lab and Fgf10 flox/flox mice [14,15] were a kind gift from Professor Suzanne L. Mansour (University of Utah, USA). Embryonic day 0.5 (E0.5) was assigned to the day when a vaginal plug was detected.…”

Section: Mice and Tamoxifen Administrationmentioning

confidence: 99%

“…To test the potential use of this line for gene inactivation studies, Fgf10 iCre/+ ; Tomato flox/flox mice were crossed with mice carrying a 'floxed' version of Fgf10 (Fgf10 flox/flox ) [14]. Cre activity was induced by tamoxifen food from E8.5 to E14.5.…”

Section: Inducible Conditional Gene Inactivationmentioning

confidence: 99%

See 2 more Smart Citations

Characterization of a novel Fibroblast growth factor 10 (Fgf10) knock-in mouse line to target mesenchymal progenitors during embryonic development

Agha¹,

Alam²,

Carraro³

et al. 2012

Pneumologie

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Fibroblast growth factor 10 (Fgf10) is a key regulator of diverse organogenetic programs during mouse development, particularly branching morphogenesis. Fgf10-null mice suffer from lung and limb agenesis as well as cecal and colonic atresia and are thus not viable. To date, the Mlcv1v-nLacZ-24 transgenic mouse strain (referred to as Fgf10 LacZ ), which carries a LacZ insertion 114 kb upstream of exon 1 of Fgf10 gene, has been the only strain to allow transient lineage tracing of Fgf10-positive cells. Here, we describe a novel Fgf10 Cre-ERT2 knock-in line (Fgf10 iCre ) in which a Cre-ERT2-IRES-YFP cassette has been introduced in frame with the ATG of exon 1 of Fgf10 gene. Our studies show that Cre-ERT2 insertion disrupts Fgf10 function. However, administration of tamoxifen to Fgf10 iCre ; Tomato flox double transgenic embryos or adult mice results in specific labeling of Fgf10-positive cells, which can be lineage-traced temporally and spatially. Moreover, we show that the Fgf10 iCre line can be used for conditional gene inactivation in an inducible fashion during early developmental stages. We also provide evidence that transcription factors located in the first intron of Fgf10 gene are critical for maintaining Fgf10 expression over time. Thus, the Fgf10 iCre line should serve as a powerful tool to explore the functions of Fgf10 in a controlled and stage-specific manner.

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Section: Discussionsupporting

confidence: 87%

Section: Mice and Tamoxifen Administrationmentioning

confidence: 99%

See 1 more Smart Citation

Characterization of a novel Fibroblast growth factor 10 (Fgf10) knock-in mouse line to target mesenchymal progenitors during embryonic development

Agha¹,

Alam²,

Carraro³

et al. 2012

Pneumologie

View full text Add to dashboard Cite

show abstract

“…Testing the hypothesis that FGF10 is a master-regulator for lung development will require both the targeted deletion of its receptor in specific progenitor cell populations and a full analysis of the gene regulatory network controlling progenitor proliferation and morphogenesis. A lung epithelial-specific deletion of Fgfr2 has been performed and the results are consistent with roles in branching, survival, and proliferation (Abler et al, 2009). As yet, there has been no attempt to build a gene regulatory network for lung morphogenesis.…”

Section: Lung Progenitors and Branching Morphogenesismentioning

confidence: 74%

The building blocks of mammalian lung development

Rawlins

2010

Developmental Dynamics

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Progress has recently been made in identifying progenitor cell populations in the embryonic lung. Some progenitor cell types have been definitively identified by lineage-tracing studies. However, others are not as well characterized and their existence is inferred on the basis of lung morphology, or mutant phenotypes. Here, I focus on lung development after the specification of the initial lung primordium. The evidence for various lung embryonic progenitor cell types is discussed and future experiments are suggested. The regulation of progenitor proliferation in the embryonic lung, and its coordinate control with morphogenesis, is also discussed. In addition, the relationship between embryonic and adult lung progenitors is considered. Developmental Dynamics 240:463-476,

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“…The lungs were cultured on E13, and, at that point, adriamycin-exposed embryonal organs were already smaller and less branched than controls. Their development remained impaired until the end of the experiment, and it is significant that Fgf10, a key mesenchymal regulator of the process of endodermal branching (19)(20)(21)(22) whose expression is delayed in mouse embryos exposed to adriamycin (23), was also downregulated in rats with EA-TEF at the end of gestation.…”

Section: Discussionmentioning

confidence: 99%

Lung hypoplasia in rats with esophageal atresia and tracheo–esophageal fistula

et al. 2012

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IntroductIon: survivors of esophageal atresia and tracheo-esophageal fistula (ea-TeF) often suffer chronic respiratory tract disease. ea-TeF results from abnormal emergence of the trachea from the foregut. This study in a rat model tests the hypothesis that primary lung maldevelopment might be a downstream consequence of this defect. results: The lung was hypoplastic in rats with ea-TeF although the histological pattern was normal. Maturation and arteriolar wall thickness were unchanged, but mesenchymal control of airway branching was weakened. This branching was deficient from embryonal day (e13) on in adriamycin-treated explants. dIscussIon: In conclusion, the lungs were hypoplastic in rats with experimental ea-TeF due to defective embryonal airway branching. however, arteriolar wall and respiratory epithelial patterns remained normal. These findings suggest that similarly defective lung development might contribute to chronic respiratory disease in ea-TeF patients. Methods: Pregnant rats received either 1.75 mg/kg i.p. adriamycin or vehicle on e7, e8, and e9. Lungs were recovered at e15, e18, and e2. Lung weight/body weight ratio, total DNa and protein, radial alveolar count, arteriolar wall thickness, lung maturity, and mesenchymal control of airway branching were assessed. e13 lungs were cultured for 72 h and explant airway branching was measured daily. For comparisons, nonparametric tests (*P < 0.05) were used.

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Conditional gene inactivation reveals roles for Fgf10 and Fgfr2 in establishing a normal pattern of epithelial branching in the mouse lung

Cited by 146 publications

References 49 publications

Characterization of a novel Fibroblast growth factor 10 (Fgf10) knock-in mouse line to target mesenchymal progenitors during embryonic development

Characterization of a novel Fibroblast growth factor 10 (Fgf10) knock-in mouse line to target mesenchymal progenitors during embryonic development

The building blocks of mammalian lung development

Lung hypoplasia in rats with esophageal atresia and tracheo–esophageal fistula

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