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First published online 26 March 2008
doi: 10.1242/dev.015495

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Wnt7b stimulates embryonic lung growth by coordinately increasing the replication of epithelium and mesenchyme

¹ Department of Molecular and Cellular Biology, Harvard Stem Cell Institute, Harvard University, Cambridge, MA 02138, USA.
² Howard Hughes Medical Institute, Massachusetts General Hospital, Boston, MA 02114, USA.
³ Department of Internal Medicine, Massachusetts General Hospital, Boston, MA 02114, USA.
⁴ Department of Internal Medicine, Department of Molecular Biology, University of Texas Southwestern Medical Center, Dallas, TX 75390, USA.
⁵ Department of Cell Biology, University of Virginia, Charlottesville, VA 22908, USA.

^* Author for correspondence (e-mail: dmelton{at}harvard.edu)

Accepted 29 February 2008

	SUMMARY

TOP SUMMARY INTRODUCTION MATERIALS AND METHODS TUNEL RESULTS DISCUSSION REFERENCES

 
The effects of Wnt7b on lung development were examined using a conditional Wnt7b-null mouse. Wnt7b-null lungs are markedly hypoplastic, yet display largely normal patterning and cell differentiation. In contrast to findings in prior hypomorphic Wnt7b models, we find decreased replication of both developing epithelium and mesenchyme, without abnormalities of vascular smooth muscle development. We further demonstrate that Wnt7b signals to neighboring cells to activate both autocrine and paracrine canonical Wnt signaling cascades. In contrast to results from hypomorphic models, we show that Wnt7b modulates several important signaling pathways in the lung. Together, these cascades result in the coordinated proliferation of adjacent epithelial and mesenchymal cells to stimulate organ growth with few alterations in differentiation and patterning.

Key words: Lung organogenesis, Wnt signaling, Organ growth

	INTRODUCTION

TOP SUMMARY INTRODUCTION MATERIALS AND METHODS TUNEL RESULTS DISCUSSION REFERENCES

 
Wnt proteins play important roles in the growth and morphogenesis of many organs. In lung, Wnt signaling has been proposed to stimulate the proliferation of undifferentiated progenitors (De Langhe et al., 2005; Mucenski et al., 2003; Okubo and Hogan, 2004; Okubo et al., 2005), to affect proximodistal patterning (Mucenski et al., 2003; Shu et al., 2005), and to regulate branching morphogenesis (Dean et al., 2005). Multiple Wnt ligands, Frizzled receptors, and endogenous inhibitors of Wnt activity including Dkk, Sfrp and Kremen proteins add to the complexity of Wnt signaling in the lung (De Langhe et al., 2005; Shu et al., 2002). As a result, no simple consensus model of Wnt action has emerged (Cardoso and Lu, 2006).

Experiments altering Wnt signaling in the lung have yielded conclusions that are difficult to reconcile. The use of Wnt ligands (Dean et al., 2005) or Wnt antagonists (De Langhe et al., 2005) in culture is likely to promiscuously modify multiple Wnt interactions, and these considerations might explain, in part, why a Wnt antagonist produces a decrease in epithelial branching (De Langhe et al., 2005), whereas the morpholino knockdown of β-catenin results in enhanced branching (Dean et al., 2005). Additionally, phenotypes in lung patterning following epithelial β-catenin deletion (Mucenski et al., 2003; Shu et al., 2005) could be a result of altered Wnt signaling or of non-signaling effects of β-catenin elimination (Dean et al., 2005). We therefore used in vivo genetic deletion of a single Wnt ligand to clarify its effect on lung development.

The distal lung bud tip is the site of greatest cell proliferation in the embryonic lung (Cardoso and Lu, 2006; Eblaghie et al., 2006; Liu and Hogan, 2002; Okubo et al., 2005; Perl et al., 2002; Rawlins and Hogan, 2006; Warburton et al., 2000). Wnt5a and Wnt7b are both expressed most highly in this location (Shu et al., 2002; Wang et al., 2005; Weidenfeld et al., 2002). Wnt5a-null mice exhibit increased cell proliferation in both epithelium and mesenchyme with a resulting expansion of the distal lung and increased lung size (Li et al., 2002). In this study, we focused on the action of Wnt7b.

A null mutation of Wnt7b deleting most of exon 3 and exon 4 (Wnt7b^D3-4, see Fig. S1 in the supplementary material) results in early placental lethality (Parr et al., 2001), precluding an analysis of its role in lung growth. A second allele, Wnt7b^lacZ, was created in which exon 1 (including the endogenous initiation codon and the predicted signal sequence) was replaced with lacZ and a PGK-Neomycin cassette (see Fig. S1 in the supplementary material). Homozygous Wnt7b^lacZ animals bypass placental lethality and are born with hypoplastic lungs (Shu et al., 2002). We generated a third allele, Wnt7b^D1, in which exon 1 (including the ATG codon and the predicted signal sequence) was deleted (see Fig. S1 in the supplementary material) (Lobov et al., 2005). Surprisingly, Wnt7b^D1 homozygotes with a genetic deletion analogous to that of the Wnt7b^lacZ homozygotes are viable and fertile, without a respiratory defect. The Wnt7b^D1 allele is obviously hypomorphic, but displays decreased in vivo Wnt-reporter activity and phenotypes associated with loss of Wnt activity (Lobov et al., 2005). We now show that the Wnt7b^D1 allele is hypomorphic due to alternative exon 1 splicing. Alternative splicing is also predicted to occur in the Wnt7b^lacZ allele. To generate an unambiguous conditional null allele, we created another mutant allele designated Wnt7b^C3 (see Fig. 1A), which conditionally deletes exon 3 when Cre recombinase is present to produce the Wnt7b^D3-null allele (Fig. 1A and see Fig. S1 in the supplementary material).

We show that Wnt7b^D3 homozygotes have markedly hypoplastic lungs. In contrast to the Wnt7b^lacZ hypomorphic lungs, the lungs of Wnt7b^D3 homozygotes display similarly decreased proliferation in both mesenchyme and epithelium throughout embryonic development. Furthermore, they possess incomplete tracheal cartilaginous rings and minor branching defects not noted in the prior hypomorphic animals. Interestingly, Wnt7b^D3 homozygous lungs manifest largely normal cell-fate specification and tissue geometry including, and in contrast to the Wnt7b^lacZ mice, normal vascular smooth muscle development. This genuine null model now reveals that Wnt7b does interact with known important lung mitogenic pathways. We further demonstrate that Wnt7b activates an autocrine epithelial and a paracrine mesenchymal canonical Wnt signaling mechanism. Together, these cascades stimulate the replication of both epithelium and mesenchyme in concert. The preservation of most aspects of cell fate differentiation and lung architecture, in the setting of profoundly decreased growth, suggest a surprising specificity in the action of Wnt7b.

	MATERIALS AND METHODS

TOP SUMMARY INTRODUCTION MATERIALS AND METHODS TUNEL RESULTS DISCUSSION REFERENCES

 
Mice
Male mice doubly heterozygous for the Sox2-Cre transgene (Hayashi et al., 2002) and the null Wnt7b^D3 allele were crossed with female mice that were homozygous for the floxed conditional allele of Wnt7b^C3. This conditional allele produces the Wnt7b^D3-null allele after Cre-mediated excision of exon 3. The details of the targeting for this allele and Wnt7b^D1 are available upon request and the complete results of an allelic series of Wnt7b mutants (T.J.C. and A.P.M., unpublished) will be presented elsewhere. All Wnt7b mutant lines were maintained on an identical (129/SvJ x SW) background. Progeny of the above cross were genotyped using the following primers: Sox2Cre Fwd, 5'-CTCTAGAGCCTCTGCTAACC-3' and Sox2Cre Rev, 5'-CCTGGCGATCCCTGAACATGTCC-3' (400 bp); Wnt7b null (Parr) Fwd, 5'-GGGGAATTCCGGGCGTGGCGCATGCTGTC-3' and Wnt7b null (Parr) Rev, 5'-GCAGGCATGCTGGGGATGCGG-3' (300 bp); Wnt7b conditional allele Fwd, 5'-TGACAGAGGATGGGGAGAAG-3' and Wnt7b conditional allele Rev, 5'-GGTCTTTCCAAGGGTGGTCT-3' (200 bp); Wnt7b exon 3 Cre-excised null allele Fwd, 5'-GAGGAAGTCAGGCAGGTGTC-3' and Wnt7b exon 3 Cre-excised null allele Rev, 5'-TATCCCACCGATACGCAAAC-3'(354 bp).

Tissue preparation
Lungs for immunohistochemistry were fixed in 4% paraformaldehyde for 1 hour at 4°C, and embedded in OCT or paraffin. For in situ hybridization (ISH), lungs were fixed overnight at 4°C. For whole-mount ISH, the lungs were dehydrated in methanol. For section ISH, lungs were dehydrated and embedded in paraffin.

In situ hybridization
Section and whole-mount ISH with digoxigenin-labeled probes was performed as previously described (Gray et al., 2004). The plasmid used to generate the Bmp4 probe was a gift from B. Hogan (Duke University, Durham, NC). Plasmids for Fgf10 and Lef1 probes were gifts from S. Bellusci (University of Southern California, Los Angeles, CA). Remaining probes were obtained from a genome-wide transcription factor library (Gray et al., 2004).

BrdU incorporation and detection
Pregnant mice received intraperitoneal injection of BrdU (Amersham Bioscience, UK) as recommended by the manufacturer. After 1 hour, lungs were harvested and fixed. The paired t-test was used to assay for proliferation and P<0.05 was considered significant.

	TUNEL

TOP SUMMARY INTRODUCTION MATERIALS AND METHODS TUNEL RESULTS DISCUSSION REFERENCES

 
Apoptosis was assayed using the Dead End Apoptosis Detection System (Promega).

Immunohistochemistry
Primary antibodies used were: rabbit anti-CC10 1:50 (Santa Cruz); rat anti-E-cadherin 1:2000 (Zymed); rabbit anti-fibronectin 1:100 (Chemicon); rabbit anti-N-myc 1:100 (Santa Cruz); rat anti-PECAM 1:100 (BD Pharmingen); mIgG_2a anti-smooth muscle actin 1:200 (Sigma); rabbit anti-smooth muscle myosin 1:100 (Biomedical Technologies); goat anti-Sox2 1:50 (Santa Cruz); goat anti-Sox9 1:50 (Santa Cruz); rabbit anti-pro-surfactant protein C (SP-C) 1:200 (Upstate); mIgG_2a anti-BrdU 1:100 (Amersham Biosciences).

Secondary antibodies were conjugated to Alexa-Fluor 568 (1:500, Invitrogen). Slides prepared for BrdU detection were treated with citrate buffer (1.8 mM citric acid, 8.2 mM sodium citrate, pH 6.0) for 10 minutes at 89°C. Slides prepared for N-myc detection were treated with 1 mM EDTA for 10 minutes at 89°C.

Cell counting
Representative images from multiple tissue samples were counted. Approximately 7500 cells were counted in the tracheal epithelium and the distal airway. For Sox9-positive cells, 868 and 869 cells were counted in mutant and wild-type lungs, respectively. For cells in the alveolar sacs, 7532 cells, evenly divided between mutant and wild-type samples, were counted. When evaluating BrdU incorporation, a total of 13,304 cells were counted. Endoderm cells surrounded by smooth muscle were counted as stalk cells, whereas more distal endoderm cells were counted as tip cells.

Explant culture
Whole lung, isolated mesenchyme (Weaver et al., 2003), and recombined endoderm and mesenchyme culture (Bellusci et al., 1997a; Weaver et al., 2000) were performed. Whole lungs were dissected at E12.5 in PBS and grown in 50% DMEM (Gibco), 50% Ham's F12 (CellGrow), with penicillin, streptomycin, and glutamine (Gibco) at 37°C for 24 to 48 hours on Nucleopore Track-Etch membrane filters (Whatman). Dkk1 at 200 ng/ml (R&D Systems), LiCl at 20 mM, and Bmp4 at 100 ng/ml (R&D Systems) were added to the media as described.

	RESULTS

TOP SUMMARY INTRODUCTION MATERIALS AND METHODS TUNEL RESULTS DISCUSSION REFERENCES

 
Wnt7b consists of two different isoforms generated by alternative exon 1 usage
Previously reported Wnt7b alleles were designed to result in a null phenotype by removing exon 1 along with its start codon and predicted signal sequence (see Fig. S1 in the supplementary material) (Lobov et al., 2005; Shu et al., 2002). However, neither of these alleles phenocopied the early lethality associated with the Wnt7b^D3-4 allele, even though Wnt7b^D1 homozygotes were on an identical background. Either the removal of exon 1 resulted in a partial loss-of-function allele, or the more severe Wnt7b^D3-4 allele acted as a dominant-negative. The presence of transcripts containing the third exon in Wnt7b^lacZ mice is consistent with the former possibility (Shu et al., 2002), and the hypothesis that the more severe Wnt7b^D3-4 allele acts as a dominant-negative allele is unlikely because heterozygous animals display no phenotype (Parr et al., 2001).

Previous studies have shown that some Wnts exist as distinct protein isoforms. To test the possibility that the Wnt7b^D1 animals are incomplete nulls due to the existence of an alternative exon 1, we performed RNase protection assays with a probe spanning exon 2 and the previously identified exon 1. This analysis suggested that there are indeed two isoforms of Wnt7b (see Fig. S2 in the supplementary material). Subsequent 5' RACE identified an alternative Wnt7b transcript that utilizes a distinct first exon with its own ATG and a highly conserved signal sequence (see Fig. S2 in the supplementary material). We identified corresponding transcripts in the NCBI nucleotide database and E14.5 lung (see Fig. S2 in the supplementary material). In Wnt7b^D1 homozygous animals, we saw upregulation of the alternative transcript (see Fig. S2 in the supplementary material). These transcripts are likely to correspond to the residual exon 3 transcripts that were present in the Wnt7b^lacZ hypomorphic mutants, strongly suggesting that alternative splicing occurs in Wnt7b^lacZ homozygotes (Shu et al., 2002). Thus, Wnt7b^D3-4 mice represent a true null phenotype, whereas the other two alleles represent a partial loss-of-function.

Generation of a conditional null allele of Wnt7b
To characterize the role of Wnt7b in the lung, we used a conditional strategy to remove Wnt7b function from the entire embryo but not the placenta. The conditional knock-in allele, Wnt7b^C3, contains loxP sites flanking exon 3, and generates the null allele Wnt7b^D3 upon Cre-mediated removal of exon 3. Wnt7b^D3 was designed to mimic the true null Wnt7b^D3-4 allele (see Fig. S1 in the supplementary material). Furthermore, Wnt7b^D3 does not retain a constitutively active promoter driving a neomycin resistance cassette, which has resulted in neomorphic effects in other systems (see Fig. S1 in the supplementary material). Germline removal of Wnt7b^D3 results in placental lethality as expected, similar to that of the original Wnt7b^D3-4 mutants. We next used a Sox2-Cre transgenic driver line (Hayashi et al., 2002), in which Cre is produced only in the epiblast, to recombine Wnt7b^C3 throughout the embryo proper, well before organogenesis. Conversely, extraembryonic tissues, including placenta, where Sox2-Cre is not expressed, retain the phenotypically wild-type Wnt7b^C3 conditional allele. Using this strategy, phenotypically normal Wnt7b^C3 homozygous mice were mated with the phenotypically normal doubly heterozygous Sox2-Cre; Wnt7b⁺Wnt7b^D3 mice (Fig. 1A). We expected 25% of pups to possess two null Wnt7b^D3 alleles (Fig. 1A). When present, Sox2-Cre expression completely converted the Wnt7b^C3 allele to Wnt7b^D3 in all E9.5 embryonic tissues (see Fig. S3 in the supplementary material).

View larger version (37K): [in this window] [in a new window]   Fig. 1. Deletion of mouse Wnt7b results in hypoplastic lungs. (A) Strategy to remove Wnt7b from only the embryo proper. (B) Mutant lungs are 50% smaller than wild-type at E18.5. The overall mass of the embryo is unchanged. (C) Mutant lungs are 75% smaller than wild-type at E14.5. The overall mass of the embryo is unchanged. (D) Control and mutant lungs at E12.5. E-cadherin staining shows grossly normal lobulation in mutant lungs. However, the right medial lobe bronchus (*) of the Wnt7b mutant lung emanates from the cephalic lobe bronchus.

At E12.5, mutant lungs were visibly smaller (Fig. 1D), but their lobar branching was largely preserved. The correct number of lobes was formed, but the medial lobe bronchus of the right lung emanated from the cephalic lobe bronchus in the Wnt7b mutant (Fig. 1D). At E14.5, mutant lungs had fewer distal tips and displayed a relative thinning of the mesenchyme (Fig. 2A-D and see Fig. S3 in the supplementary material). A wild-type E14.5 lung has 1000 distal tips abutting the mesothelium, whereas the mutant lung had 500 tips. The trachea appeared normal in diameter and length with an intact epithelium and normal smooth muscle. However, in contrast to Wnt7b^lacZ mice, the cartilaginous rings of the trachea were incomplete (data not shown).

Normal cell differentiation and patterning are preserved in Wnt7b-null lungs
We next examined cell fate differentiation both qualitatively and quantitatively. At E14.5, normally distributed networks of PECAM (Pecam1)-positive endothelial cells are present in the proximal and distal lung (Fig. 2A). Smooth muscle surrounds the proximal airways and vasculature and was appropriately absent around distal tip endoderm (Fig. 2B). The proximal airway marker Sox2 was expressed appropriately in the trachea and proximal airways and was excluded from distal endoderm (Fig. 2C), whereas Sox9 was appropriately expressed in the distal tip endoderm and excluded proximally (Fig. 2D).

Normal differentiation and patterning were also seen at E18.5 (Fig. 2E-H). Blood vessels adopted characteristic vascular networks (Fig. 2E) and smooth muscle surrounded proximal airways and blood vessels (Fig. 2F). We found no evidence of vascular smooth muscle abnormality, including previously described hypertrophy or apoptosis (see Fig. S4 in the supplementary material) (Shu et al., 2002). CC10 (Scgb1a1 - Mouse Genome Informatics), a proximal epithelial marker, was present in the airways and was appropriately absent distal to the bronchoalveolar duct junction (Fig. 2G). Finally, type 2 cells expressing SP-C (Sftpc - Mouse Genome Informatics) occurred in the distal saccules (Fig. 2H), whereas type 1 cells were present in decreased numbers in the alveoli (Fig. 2I).

At E18.5, Clara cells, ciliated cells, and mucous cells each were present in their usual ratios (Fig. 2J). Mucous cells were appropriately absent in Wnt7b mutant bronchi. Even the subtle increase in the relative percentage of ciliated cells to Clara cells that is normally seen in bronchi as compared with trachea (Fig. 2J), occurred normally in mutant lungs (Fig. 2J). At E18.5, SP-C-positive type 2 cells comprised 37% of the cells in both wild-type and mutant lungs (Fig. 2J). The percentage of PECAM-staining cells was not significantly altered, comprising 49% of total cells in controls and 46% in mutant lungs (Fig. 2J). The filamentous staining of type 1 cells for caveolin 1 precluded rigorous quantitation, but a qualitative reduction in type 1 cell number was seen. Finally, we quantified the number of distal epithelial progenitor cells per tip by counting Sox9-positive cells at E14.5 (Liu and Hogan, 2002; Okubo et al., 2005). We found that the number of Sox9-positive cells per lung bud tip was unchanged, with a mean of 24 cells per tip on cross-section (Fig. 2K). However, as the Wnt7b mutant lung contains fewer lung bud tips, the total number of epithelial progenitor cells in the mutant lung is reduced.

View larger version (89K): [in this window] [in a new window]   Fig. 2. Cell fate specification, timing of differentiation and tissue architecture are unchanged in Wnt7b-null lungs. (A-D') E14.5 immunohistochemistry of heterozygous (A-D) and Wnt7b mutant (A'-D') mouse lungs. Blood vessels appear normal in the mutant, as marked by PECAM (A,A'), as does airway smooth muscle, marked by smooth muscle myosin (B,B'). Proximal Sox2 (C,C') and distal Sox9 (D,D') expression are unchanged in mutants. Dotted lines encircle the epithelium. (E-I') At E18.5, immunohistochemistry of heterozygous (E-I) and Wnt7b mutant (E'-I') lungs demonstrates that blood vessels (E,E'), airway smooth muscle cells (F,F'), Clara cells as marked by CC10 (G,G'), and type 2 cells as marked by surfactant protein C (H,H') are unchanged in mutant lungs. Type 1 cells marked by caveolin 1 (I,I') are decreased in number. (J) Quantification of cell types in E18.5 lungs demonstrates that the proportions of Clara, ciliated and mucous cells are unchanged in the trachea and airways of Wnt7b mutants. In the distal saccules, the proportions of cells positive for SP-C or PECAM are also unchanged. Error bars represent 1 s.d. (K) The number of Sox9-positive cells per lung bud tip at E14.5 is unchanged in Wnt7b mutants.

To further characterize the differentiation and patterning in the Wnt7b mutant lung, we analyzed the expression of a panel of factors chosen for their distinct expression patterns within the developing lung. A genome-scale ISH screen was performed with E14.5 embryonic mouse lungs using a recently developed transcription factor library that includes 1100 mouse transcription factors (Gray et al., 2004; Zhou et al., 2007). We identified transcription factors with distinct expression patterns during normal lung organogenesis. The expression of a subset of these genes with stereotyped patterns was compared in Wnt7b mutant and wild-type lungs. Their expression in the mutant was found to be normal (see Fig. S5 in the supplementary material). This analysis included genes expressed predominantly in distal endoderm at E14.5 (Etv5, Spry2, Foxa1, Foxa2 and Foxp4), in proximal endoderm stalks (Sox2 and Foxj1), pulmonary artery (Epas1), distal endothelial cells (Heyl), cartilaginous rings (Sox5long, Sox9, Irx2) and smooth muscle (Tgfb1i1). Genes identified as pan-mesenchymal [Hoxa2, Hoxb5, Pod1 (Tcf21) and Osr1] or periendodermal (Foxf1, Gli2 and Tbx4) were also expressed normally in mutant lungs. All these results are consistent with the general finding that Wnt7b mutant lungs are small but patterned normally.

View larger version (45K): [in this window] [in a new window]   Fig. 3. Deletion of Wnt7b results in proportionate decreases in replication of epithelial and mesenchymal tip cells. (A,A') Schematic depiction (A') of BrdU staining (brown) of E14.5 lung bud tip (A). Replication is highest in tip epithelium (A', dark yellow) and tip mesenchyme (A', dark purple) as compared with proximal epithelium (A', light yellow) and mesenchyme (A', light purple). (B,C) TUNEL staining of E14.5 wild-type (B) and Wnt7b mutant (C) mouse lungs shows no increase in apoptosis in the mutant. Dotted lines encircle epithelium. (D,E) BrdU staining of E14.5 wild-type (D) and mutant (E) lungs demonstrates decreased replication in mesenchymal and epithelial cells of the mutant. Arrowheads point to the tips. Dotted lines encircle epithelium. (F) A comparison of the percentage of BrdU-labeled cells in wild-type (gray) and mutant (white) tips demonstrates proportionate drops in epithelial and mesenchymal replication (P<0.001).

Many signaling pathways that modulate cell replication and differentiation are unchanged in Wnt7b-null lungs
Hypomorphic Wnt7b^lacZ homozygote lungs displayed no abnormalities of growth factor expression, suggesting that Wnt7b acts independently of other signaling cascades known to regulate lung development (Shu et al., 2002). We revisited growth factor expression in Wnt7b-null lungs. Since sonic hedgehog (Shh) exerts a proliferative effect on mesenchyme (Weaver et al., 2003), we examined Wnt7b-null lungs for evidence of aberrant hedgehog (Hh) signaling. Expression of Shh was confined to the endoderm of the mutant lung in a normal pattern (Fig. 4A and see Fig. S5 in the supplementary material). Gli1, a Shh target gene, was also expressed normally in the periendodermal mesenchyme (Fig. 4B and see Fig. S5 in the supplementary material). Ptch1 and Hip1 were also expressed normally (Chuang and McMahon, 1999) (Fig. 4C and see Fig. S5 in the supplementary material), as was Foxf1, a mesenchymal target of Shh (data not shown). Similarly, Fgf9, which is upstream of Shh signaling (White et al., 2006), was properly expressed in the mesothelium and the endoderm tips (see Fig. S5 in the supplementary material). Finally, mesenchymal Bmp4 expression, which is modulated by Shh signaling (Bitgood and McMahon, 1995; Weaver et al., 2000), was unchanged in the Wnt7b mutant (Fig. 5F and see Fig. S5 in the supplementary material). We conclude that Shh signaling is not altered in Wnt7b mutant lungs. This is consistent with the observed normal distribution of smooth muscle, which is altered in the absence of Hh signaling (Pepicelli et al., 1998). Conversely, studies have demonstrated that Wnt7b expression is not altered in lung mutants with diminished Hh signaling (Chuang and McMahon, 1999; Pepicelli et al., 1998). Therefore, we conclude that Wnt7b and Hh signaling are independent pathways to regulate mesenchymal cell proliferation in the embryonic lung (Chuang and McMahon, 1999; Pepicelli et al., 1998).

We next examined the expression of Fgf10, an epithelial mitogen and a regulator of branch outgrowth (Bellusci et al., 1997b; Sekine et al., 1999; Weaver et al., 2000). Wnt7b mutants demonstrated a modest, variable decrease of Fgf10 expression in the interbud distal mesenchyme, with preserved proximal mesenchymal expression (Fig. 4D and see Fig. S5 in the supplementary material). However, the expression of Spry2, a known epithelial target and antagonist of mesenchymal Fgf10 signaling (Mailleux et al., 2001), was expressed normally in the distal tip epithelium (Fig. 4E). The expression of other Wnt genes and Dkk1 was also unchanged in Wnt7b mutant lungs (see Fig. S5 in the supplementary material; data not shown). N-myc (Mycn - Mouse Genome Informatics), which is proposed to be a Wnt target, regulates the proliferation and differentiation of distal lung epithelial progenitors (Okubo et al., 2005). However, N-myc protein expression was normal in mutant lungs (Fig. 4F). Fibronectin, which has also been identified as a downstream target of canonical Wnt signaling (De Langhe et al., 2005), was deposited similarly in mutant and control lungs (Fig. 4G).

View larger version (46K): [in this window] [in a new window]   Fig. 4. Preserved expression of many factors affecting growth in Wnt7b mutant lungs. (A-E') E14.5 ISH of Wnt7b mutant (A'-E') and control (A-E) mouse lungs. Expression of Shh (A,A'), Gli1 (B,B'), Ptch1 (C,C') and Spry2 (E,E') are unchanged in the mutant. The epithelial tip is encircled. Fgf10 staining (D,D') is largely preserved in mutant lungs; there is a variable decrease in the most-distal expression of Fgf10 in mutant lungs (arrowhead). (F-G') E14.5 immunohistochemistry for N-myc (F,F') and fibronectin expression (G,G') showing that these are unchanged in the mutant. ISH signal (purple) is indicated by the arrowheads.

Epithelial Wnt7b sends a paracrine canonical signal to adjacent mesenchyme cells
To test the hypothesis that mesenchyme responds to a canonical Wnt signal, we employed organ culture. E12.5 embryonic lungs grown at an air-liquid interface exhibited normal Axin2 and Lef1 expression (Fig. 5B). Lungs with recombinant Dkk1, which has previously been shown to downregulate canonical Wnt signaling in lung bud culture (De Langhe et al., 2005), displayed reduced Axin2 and Lef1 expression. Lungs cultured with lithium to stimulate canonical Wnt signaling showed upregulated Axin2 and Lef1 expression through much of the distal mesenchyme (Fig. 5B). The ectopic expression of these Wnt target genes, which are normally restricted to the periendodermal mesenchyme, suggests that the mesenchyme is broadly competent to transduce a canonical Wnt signal.

To further test the hypothesis that the mesenchyme responds to an endodermal signal, we performed tissue recombination. When dissected mesenchyme was cultured in isolation, there was no expression of canonical Wnt target genes (Fig. 5C). When dissected epithelial buds were reaggregated with isolated mesenchyme, the endoderm and mesoderm reassociated and branching morphogenesis resumed. When recombined endoderm-mesenchyme cultures were analyzed, Wnt target gene expression was restored in periendodermal mesenchyme (Fig. 5C), confirming that endoderm is the origin of a canonical Wnt signal.

We next examined Wnt7b mutant lungs. As anticipated, these lungs did not express Axin2 or Lef1 (Fig. 5D). However, when lithium was added, the expression of these Wnt target genes was restored (Fig. 5D). Thus, Wnt7b signals directly to adjacent competent mesenchyme through a canonical Wnt signaling pathway and is responsible for the periendodermal expression of Wnt target genes in the mesenchyme immediately adjacent to the growing distal tip epithelium. This is consistent with prior reports showing that mesenchymal Fzd1 binds Wnt7b, and that Wnt7b can act through the canonical pathway (Wang et al., 2005). Since the mesenchyme seems broadly competent to receive a canonical Wnt signal, we suggest that the short range of action of Wnt7b creates a zone of induction in the periendodermal cells, which correspond to the most actively dividing mesenchymal progenitors (Fig. 3A, Fig. 5E). Coupled with the normal expression of the mesenchymal mitogens Shh and Fgf9, this is consistent with a direct mitogenic effect of Wnt7b on the lung mesenchyme.

View larger version (65K): [in this window] [in a new window]   Fig. 5. Mechanism of Wnt7b action in mouse lung development. (A) ISH showing loss of canonical Wnt targets in mesenchyme and endoderm of Wnt7b mutant lungs. Dotted lines encircle epithelium. Arrowheads point to periendodermal mesenchyme. (B) E12.5 whole-mount ISH of Axin2 and Lef1 in cultured wild-type lungs. Wnt signaling is decreased with the addition of Dkk1 (left) and enhanced by lithium (right) when compared with control cultures (middle). In lithium-treated lungs, mesenchymal staining of the canonical targets has expanded. (C) Axin2 expression in mesenchyme cultured alone and in mesenchyme recombined with epithelium, showing that mesenchymal Axin2 expression requires endoderm induction. (D) Lithium rescues Lef1 expression in E12.5 mutant lungs when compared with Wnt7b mutant lungs cultured without lithium. (E) Epithelial Wnt7b activates a canonical pathway in neighboring mesenchyme. (F) Bmp4 and Id2 expression are coincident on serial sections of E14.5 wild-type lung (left). Expression of epithelial Bmp4 and Id2 are decreased in mutant lungs (middle and right). (G) Lithium induces ectopic Id2 expression in cultured E12.5 wild-type lungs. (H) Wnt7b induces Bmp4 and Id2 production in endoderm tip cells. (I) Wnt7b coordinately activates autocrine and paracrine signaling cascades to increase cell replication.

Canonical Wnt signaling has previously been demonstrated to be upstream of epithelial Bmp4 expression (Shu et al., 2005). We sought to confirm the hypothesis that Id2 is also an endodermal Wnt target. Cultured wild-type lungs expressed Id2 only in the most distal epithelium (Fig. 5G). However, when lithium was added, Id2 expression at the distal tip was upregulated (Fig. 5G). In addition, ectopic production of Id2 occurred in proximal endoderm (Fig. 5G). Interestingly, addition of Bmp4 protein to the culture medium does not lead to an increase in Id2 expression, although Bmp4 does produce characteristic changes in bud morphology (data not shown). This suggests that Id2 expression is not downstream of Bmp4 signaling. The decrease in Id2 and Bmp4 expression in Wnt7b mutant lungs identifies Wnt7b as the source of an autocrine canonical signal (Fig. 5H). Bmp4 has been shown to act as an autocrine regulator of distal endoderm progenitor cell replication (Eblaghie et al., 2006). Thus, the decrease in Bmp4 expression explains, at least in part, the decreased rate of epithelial proliferation observed in Wnt7b-null lungs.

	DISCUSSION

TOP SUMMARY INTRODUCTION MATERIALS AND METHODS TUNEL RESULTS DISCUSSION REFERENCES

 
Analysis of the null Wnt7b^D3 allele reveals previously unappreciated functions of Wnt7b in lung development
We show that a prior model of Wnt7b deletion, using the Wnt7b^D1 allele (Lobov et al., 2005), is hypomorphic due to the presence of an alternative exon 1. Based on the presence of Wnt7b-exon-3-containing mRNA transcripts in the Wnt7b^lacZ model, this allele is likely to display alternative exon 1 splicing, as would be predicted on the basis of its genomic sequence. We further note that the Wnt7b^lacZ allele retains a constitutive promoter and neomycin resistance cassette that is not present in the Wnt7b^D3 allele. In fact, the presence of this cassette in a prior version of the Wnt7b^D1 allele caused early E9.5 embryonic lethality (distinct from and earlier than the placental abnormalities found in Wnt7b-null mice with cardiovascular and anteroposterior patterning abnormalities; data not shown). This neomorphic phenotype was completely eliminated by removing the constitutive promoter and neomycin cassette. In addition, we identified the presence of an unannotated cDNA (Unigene accession #Mm.394884), the 5' sequence of which overlaps in opposite orientation with Wnt7b exon 1. An alteration of this gene product or a neomorphic effect of the neomycin resistance cassette could account for elements of the phenotype of Wnt7b^lacZ animals, most notably the vascular smooth muscle abnormalities that are not seen in true null Wnt7b^D3 animals (Shu et al., 2002).

Analysis of the lungs of Wnt7b^D3 homozygotes reveals a number of new findings, including a reduction in the replication of both epithelium and mesenchyme, in contrast to the previously reported reduction in mesenchyme proliferation (Shu et al., 2002). Additionally, we demonstrate defects in tracheal cartilage formation and minor branching abnormalities not seen in Wnt7b^lacZ homozygotes. Most importantly, a characterization of the lung hypoplasia in these true null mice demonstrates that Wnt7b interacts with known signaling cascades in the lung and activates a canonical signaling cascade in both mesenchyme and epithelium. The analysis of the hypomorphic Wnt7b^lacZ animals, by contrast, demonstrated no such interactions, implying that Wnt7b was independent of these signaling pathways.

Importantly, we see no abnormalities in smooth muscle development or apoptosis as previously noted in Wnt7b^lacZ animals (Shu et al., 2002). The greater large vessel hemorrhage seen in these animals was likely to have been potentiated by smooth muscle irregularity and apoptosis. In Wnt7b^D3 true null animals, small vessel and large vessel hemorrhage occur with equal frequency, and are likely to be a consequence of the pulmonary hypertension that results from vascular hypoplasia in the setting of normal cardiac size.

A decrease in replication of epithelium and mesenchyme in Wnt7b mutants results in a small lung with preserved differentiation and architecture
Wnt signaling in the lung has been proposed to modulate the behavior of distal progenitor cells (Cardoso and Lu, 2006; Perl et al., 2002; Warburton et al., 2000). Wnts have been proposed to stimulate the replication of tip progenitors, to inhibit the differentiation of tip progenitors, and to modulate tip progenitors to alter the ratio of proximal to distal cell differentiation (Cardoso and Lu, 2006; De Langhe et al., 2005; Liu and Hogan, 2002; Mucenski et al., 2003; Okubo and Hogan, 2004; Okubo et al., 2005; Weaver et al., 2000). The hypoplastic phenotype of Wnt7b^D3 homozygous animals is caused by a similar decrease in proliferation of both epithelium and mesenchyme, resulting in the diminished production of differentiated cells, which, nonetheless, largely retain their normal patterning and tissue geometry. Interestingly, the number of Sox9-positive epithelial progenitors within a given lung bud tip does not change. Surprisingly, the time-course of differentiation proceeds normally despite this decrease in cell division. This suggests that the mechanisms regulating the timing of cell differentiation can be partly uncoupled from the mechanisms that regulate cell replication.

Epithelial Wnt7b activates an autocrine and a paracrine canonical signaling cascade in adjacent pools of endoderm and mesenchyme
Wnt7b induces a canonical Wnt signaling cascade in adjacent epithelium and mesenchyme. Previous studies using Wnt-reporter lines did not demonstrate canonical Wnt reception within the mesenchyme (De Langhe et al., 2005; Dean et al., 2005; Okubo and Hogan, 2004; Shu et al., 2005). However, the mesenchymal expression of the Wnt target genes Axin2 and Lef1 (Jho et al., 2002; Tebar et al., 2001), and mesenchymal β-catenin staining (Shu et al., 2005; Tebar et al., 2001), have been previously noted. We now show that lung mesenchyme is broadly competent to transduce a canonical Wnt signal, and suggest that the periendodermal restriction of canonical Wnt activity is due to a local action of Wnt7b (Lobov et al., 2005). As Wnt-reporter mice do not capture the entire array of Wnt signaling events (Dean et al., 2005; He et al., 2004), it will be of interest to re-examine reports of altered Wnt signaling in the lung in light of this new finding.

Wnt7b also activates a canonical signaling cascade in the endoderm to induce the expression of Bmp4 and Id2. Our findings are consistent with prior work that establishes that Wnt signaling is upstream of Bmp4 (Shu et al., 2005) and that Wnt7b is able to transduce a canonical Wnt signal in vitro (Wang et al., 2005). Bmp4 signaling regulates the proliferation of distal tip epithelial cells (Eblaghie et al., 2006), and we suggest that Wnt7b, at least in part, stimulates the autocrine amplification of progenitor cell replication through this mechanism. Id2 is also known to stimulate cell proliferation in many contexts (Kowanetz et al., 2004; Lasorella et al., 2002; Memezawa et al., 2007; Nigten et al., 2005; Yokota et al., 2001) and is located downstream of Bmp4 in other systems (Hollnagel et al., 1999; Hua et al., 2006; Ying et al., 2003). Our preliminary in vitro experiments suggest, however, that in lung epithelium, Bmp4 and Id2 might be parallel rather than serial targets of Wnt signaling. Further experiments will be necessary to clarify the epistatic relationships of Id2 and Bmp4 as well as the precise function of Id2, as Id2-null mice do not display an overt pulmonary phenotype (Yokota et al., 1999; Yokota et al., 2000). Efforts to phenotypically rescue Wnt7b-null lungs in culture with Fgf10 protein, Bmp4 protein, and Wnt7b-expressing cell lines were difficult to interpret owing to variable rates and patterns of BrdU incorporation in embryonic lungs grown in vitro. In summary, we propose that Wnt7b produced in the distal lung bud epithelium induces signaling cascades in both tip epithelial progenitors and adjacent mesenchyme (Fig. 5I). We hypothesize that the previously described short range of action of Wnt7b (Lobov et al., 2005) causes it, at least in part, to delimit the populations of greatest replicative activity in the embryonic lung to adjacent pools of cells located in the distal lung bud tip.

Wnt7b and lung size
The loss of Wnt7b results in the decreased replication of both epithelium and mesenchyme without grossly perturbing cell differentiation or lung architecture. This surprisingly specific result contrasts with the hypoplastic phenotypes associated with the deletion of many mitogenic factors, such as Shh, which also act to modify cell fate. Given the Wnt7b phenotype, it is therefore not surprising that Hh signaling is unchanged in Wnt7b-null lungs. Similarly, in the epithelium, Wnt7b expression results in a highly localized increase of only epithelial Bmp4 expression. More profound alterations in either Bmp or Wnt signaling might be predicted to cause changes in cell fate, based on prior observations (Okubo and Hogan, 2004; Weaver et al., 2000; Weaver et al., 1999). We speculate that such subtle modulation of mitogenic activity might be a characteristic of molecules that result in changes in growth without large effects on differentiation.

The Fgf9-null mouse is the only other mutant animal to display such profound growth defects in the absence of significant patterning abnormalities (Colvin et al., 2001). Although Fgf9 may have a disproportionate effect on mesenchyme proliferation (Colvin et al., 2001), reports do suggest that Fgf9 can also stimulate epithelial proliferation and alter smooth muscle and vascular development (del Moral et al., 2006; White et al., 2007; White et al., 2006). Fgf9 expression, however, remains normal in Wnt7b-null mice (see Fig. S5 in the supplementary material; data not shown). Furthermore, Wnt7b-null mice display entirely normal Hh signaling, and this pathway is modulated by Fgf9 and is responsible for many of its mitogenic actions on the mesenchyme (White et al., 2006). Interestingly, both Wnt7b- and Fgf9-null mutants display decreased Fgf10 expression in the distal interbud region, with preservation of more proximal Fgf10 expression (Fig. 4D and see Fig. S5 in the supplementary material) (White et al., 2006). Future experiments should examine the interaction of Wnt7b and Fgf9 and their precise relationships to the Bmp4, Shh and Fgf10 cascades. Indeed, the regulation of Wnt antagonists such as Dkk1 can be induced by Fgf9, and may play a role in limiting lung size by antagonizing Wnt7b (De Langhe et al., 2005; del Moral et al., 2006). Similarly, Wnt5a, a non-canonical Wnt, may antagonize Wnt7b function to limit lung growth (De Langhe et al., 2005; Li et al., 2002).

Finally, it is unclear whether lung growth is proportional to Wnt7b dose, or whether there is a threshold level beneath which lung size drops precipitously. Preliminary observations on a set of allelic crosses conducted on an identical genetic background show that mice that possess one Wnt7b^D1 and one Wnt7b^D3-4 allele possess an intermediate phenotype, with incomplete tracheal cartilaginous rings but normally sized lungs. This suggests the possibility that the tracheal phenotype is more sensitive to loss of Wnt7b exon 1a than is the lung size phenotype. Unfortunately, we find no combination of alleles that results in graded changes in lung growth. The current lack of understanding of the distinct roles and expression patterns of the two alternatively spliced Wnt7b isoforms clouds interpretation. It is unlikely that the Wnt7b^lacZ allele will contribute meaningfully to an allelic series of mutants as Wnt7b^lacZ undergoes not only alternative splicing, but also displays a neomorphic phenotype. However, a complete analysis of the remaining combination of alleles on a common background should help clarify the roles of different splice forms of Wnt7b. Since Wnt7b protein has evaded purification, we propose that a genetic model permitting finely regulable, graded Wnt7b expression on a Wnt7b^D3-null background would permit an analysis of the exact effect of Wnt7b on lung size.

Supplementary material
Supplementary material for this article is available at http://dev.biologists.org/cgi/content/full/135/9/1625/DC1

	ACKNOWLEDGMENTS

 
We thank Saverio Bellusci, Brigid Hogan, Ed Morrisey, David Ornitz and Jeff Whitsett for discussion and plasmids; Renate Hellmiss for her expertise in figure design; and Justin Annes, Yuval Dor, Amy Greenwood and Ben Stanger for sharing their insights about size regulation. D.A.M. is an HHMI Investigator. A.P.M. is supported by NIDDK 054364. J.R. is supported by NHLBI HL076393.

	REFERENCES

TOP SUMMARY INTRODUCTION MATERIALS AND METHODS TUNEL RESULTS DISCUSSION REFERENCES

 

Bellusci, S., Furuta, Y., Rush, M. G., Henderson, R., Winnier, G. and Hogan, B. L. (1997a). Involvement of Sonic hedgehog (Shh) in mouse embryonic lung growth and morphogenesis. Development 124,53 -63.[Abstract]
Bellusci, S., Grindley, J., Emoto, H., Itoh, N. and Hogan, B. L. (1997b). Fibroblast growth factor 10 (FGF10) and branching morphogenesis in the embryonic mouse lung. Development 124,4867 -4878.[Abstract]
Bitgood, M. J. and McMahon, A. P. (1995). Hedgehog and Bmp genes are coexpressed at many diverse sites of cell-cell interaction in the mouse embryo. Dev. Biol. 172,126 -138.[CrossRef][Medline]
Cardoso, W. V. and Lu, J. (2006). Regulation of early lung morphogenesis: questions, facts and controversies. Development 133,1611 -1624.[Abstract/Free Full Text]
Chuang, P. T. and McMahon, A. P. (1999). Vertebrate Hedgehog signalling modulated by induction of a Hedgehog-binding protein. Nature 397,617 -621.[CrossRef][Medline]
Colvin, J. S., White, A. C., Pratt, S. J. and Ornitz, D. M. (2001). Lung hypoplasia and neonatal death in Fgf9-null mice identify this gene as an essential regulator of lung mesenchyme. Development 128,2095 -2106.[Abstract/Free Full Text]
De Langhe, S. P., Sala, F. G., Del Moral, P. M., Fairbanks, T. J., Yamada, K. M., Warburton, D., Burns, R. C. and Bellusci, S. (2005). Dickkopf-1 (DKK1) reveals that fibronectin is a major target of Wnt signaling in branching morphogenesis of the mouse embryonic lung. Dev. Biol. 277,316 -331.[CrossRef][Medline]
Dean, C. H., Miller, L. A., Smith, A. N., Dufort, D., Lang, R. A. and Niswander, L. A. (2005). Canonical Wnt signaling negatively regulates branching morphogenesis of the lung and lacrimal gland. Dev. Biol. 286,270 -286.[CrossRef][Medline]
del Moral, P. M., De Langhe, S. P., Sala, F. G., Veltmaat, J. M., Tefft, D., Wang, K., Warburton, D. and Bellusci, S. (2006). Differential role of FGF9 on epithelium and mesenchyme in mouse embryonic lung. Dev. Biol. 293, 77-89.[CrossRef][Medline]
Eblaghie, M. C., Reedy, M., Oliver, T., Mishina, Y. and Hogan, B. L. (2006). Evidence that autocrine signaling through Bmpr1a regulates the proliferation, survival and morphogenetic behavior of distal lung epithelial cells. Dev. Biol. 291, 67-82.[CrossRef][Medline]
Gray, P. A., Fu, H., Luo, P., Zhao, Q., Yu, J., Ferrari, A., Tenzen, T., Yuk, D. I., Tsung, E. F., Cai, Z. et al. (2004). Mouse brain organization revealed through direct genome-scale TF expression analysis. Science 306,2255 -2257.[Abstract/Free Full Text]
Hayashi, S., Lewis, P., Pevny, L. and McMahon, A. P. (2002). Efficient gene modulation in mouse epiblast using a Sox2Cre transgenic mouse strain. Mech. Dev. 119 Suppl. 1,S97 -S101.
He, X. C., Zhang, J., Tong, W. G., Tawfik, O., Ross, J., Scoville, D. H., Tian, Q., Zeng, X., He, X., Wiedemann, L. M. et al. (2004). BMP signaling inhibits intestinal stem cell self-renewal through suppression of Wnt-beta-catenin signaling. Nat. Genet. 36,1117 -1121.[CrossRef][Medline]
Hogan, B. L. (1999). Morphogenesis. Cell 96,225 -233.[CrossRef][Medline]
Hollnagel, A., Oehlmann, V., Heymer, J., Ruther, U. and Nordheim, A. (1999). Id genes are direct targets of bone morphogenetic protein induction in embryonic stem cells. J. Biol. Chem. 274,19838 -19845.[Abstract/Free Full Text]
Hua, H., Zhang, Y. Q., Dabernat, S., Kritzik, M., Dietz, D., Sterling, L. and Sarvetnick, N. (2006). BMP4 regulates pancreatic progenitor cell expansion through Id2. J. Biol. Chem. 281,13574 -13580.[Abstract/Free Full Text]
Jho, E. H., Zhang, T., Domon, C., Joo, C. K., Freund, J. N. and Costantini, F. (2002). Wnt/beta-catenin/Tcf signaling induces the transcription of Axin2, a negative regulator of the signaling pathway. Mol. Cell. Biol. 22,1172 -1183.[Abstract/Free Full Text]
Kowanetz, M., Valcourt, U., Bergstrom, R., Heldin, C. H. and Moustakas, A. (2004). Id2 and Id3 define the potency of cell proliferation and differentiation responses to transforming growth factor beta and bone morphogenetic protein. Mol. Cell. Biol. 24,4241 -4254.[Abstract/Free Full Text]
Lasorella, A., Boldrini, R., Dominici, C., Donfrancesco, A., Yokota, Y., Inserra, A. and Iavarone, A. (2002). Id2 is critical for cellular proliferation and is the oncogenic effector of N-myc in human neuroblastoma. Cancer Res. 62,301 -306.[Abstract/Free Full Text]
Li, C., Xiao, J., Hormi, K., Borok, Z. and Minoo, P. (2002). Wnt5a participates in distal lung morphogenesis. Dev. Biol. 248,68 -81.[CrossRef][Medline]
Liu, Y. and Hogan, B. L. (2002). Differential gene expression in the distal tip endoderm of the embryonic mouse lung. Gene Expr. Patterns 2,229 -233.[CrossRef][Medline]
Lobov, I. B., Rao, S., Carroll, T. J., Vallance, J. E., Ito, M., Ondr, J. K., Kurup, S., Glass, D. A., Patel, M. S., Shu, W. et al. (2005). WNT7b mediates macrophage-induced programmed cell death in patterning of the vasculature. Nature 437,417 -421.[CrossRef][Medline]
Mailleux, A. A., Tefft, D., Ndiaye, D., Itoh, N., Thiery, J. P., Warburton, D. and Bellusci, S. (2001). Evidence that SPROUTY2 functions as an inhibitor of mouse embryonic lung growth and morphogenesis. Mech. Dev. 102,81 -94.[CrossRef][Medline]
Memezawa, A., Takada, I., Takeyama, K., Igarashi, M., Ito, S., Aiba, S., Kato, S. and Kouzmenko, A. P. (2007). Id2 gene-targeted crosstalk between Wnt and retinoid signaling regulates proliferation in human keratinocytes. Oncogene 26,5038 -5045.[CrossRef][Medline]
Mucenski, M. L., Wert, S. E., Nation, J. M., Loudy, D. E., Huelsken, J., Birchmeier, W., Morrisey, E. E. and Whitsett, J. A. (2003). beta-Catenin is required for specification of proximal/distal cell fate during lung morphogenesis. J. Biol. Chem. 278,40231 -40238.[Abstract/Free Full Text]
Nigten, J., Breems-de Ridder, M. C., Erpelinck-Verschueren, C. A., Nikoloski, G., van der Reijden, B. A., van Wageningen, S., van Hennik, P. B., de Witte, T., Lowenberg, B. and Jansen, J. H. (2005). ID1 and ID2 are retinoic acid responsive genes and induce a G0/G1 accumulation in acute promyelocytic leukemia cells. Leukemia 19,799 -805.[CrossRef][Medline]
Okubo, T. and Hogan, B. L. (2004). Hyperactive Wnt signaling changes the developmental potential of embryonic lung endoderm. J. Biol. 3,11 .[CrossRef][Medline]
Okubo, T., Knoepfler, P. S., Eisenman, R. N. and Hogan, B. L. (2005). Nmyc plays an essential role during lung development as a dosage-sensitive regulator of progenitor cell proliferation and differentiation. Development 132,1363 -1374.[Abstract/Free Full Text]
Parr, B. A., Cornish, V. A., Cybulsky, M. I. and McMahon, A. P. (2001). Wnt7b regulates placental development in mice. Dev. Biol. 237,324 -332.[CrossRef][Medline]
Pepicelli, C. V., Lewis, P. M. and McMahon, A. P. (1998). Sonic hedgehog regulates branching morphogenesis in the mammalian lung. Curr. Biol. 8,1083 -1086.[CrossRef][Medline]
Perl, A. K., Wert, S. E., Nagy, A., Lobe, C. G. and Whitsett, J. A. (2002). Early restriction of peripheral and proximal cell lineages during formation of the lung. Proc. Natl. Acad. Sci. USA 99,10482 -10487.[Abstract/Free Full Text]
Rawlins, E. L. and Hogan, B. L. (2006). Epithelial stem cells of the lung: privileged few or opportunities for many? Development 133,2455 -2465.[Abstract/Free Full Text]
Sekine, K., Ohuchi, H., Fujiwara, M., Yamasaki, M., Yoshizawa, T., Sato, T., Yagishita, N., Matsui, D., Koga, Y., Itoh, N. et al. (1999). Fgf10 is essential for limb and lung formation. Nat. Genet. 21,138 -141.[CrossRef][Medline]
Shu, W., Jiang, Y. Q., Lu, M. M. and Morrisey, E. E. (2002). Wnt7b regulates mesenchymal proliferation and vascular development in the lung. Development 129,4831 -4842.[Medline]
Shu, W., Guttentag, S., Wang, Z., Andl, T., Ballard, P., Lu, M. M., Piccolo, S., Birchmeier, W., Whitsett, J. A., Millar, S. E. et al. (2005). Wnt/beta-catenin signaling acts upstream of N-myc, BMP4, and FGF signaling to regulate proximal-distal patterning in the lung. Dev. Biol. 283,226 -239.[CrossRef][Medline]
Tebar, M., Destree, O., de Vree, W. J. and Ten Have-Opbroek, A. A. (2001). Expression of Tcf/Lef and sFrp and localization of beta-catenin in the developing mouse lung. Mech. Dev. 109,437 -440.[CrossRef][Medline]
Wang, Z., Shu, W., Lu, M. M. and Morrisey, E. E. (2005). Wnt7b activates canonical signaling in epithelial and vascular smooth muscle cells through interactions with Fzd1, Fzd10, and LRP5. Mol. Cell. Biol. 25,5022 -5030.[Abstract/Free Full Text]
Warburton, D., Schwarz, M., Tefft, D., Flores-Delgado, G., Anderson, K. D. and Cardoso, W. V. (2000). The molecular basis of lung morphogenesis. Mech. Dev. 92, 55-81.[CrossRef][Medline]
Weaver, M., Yingling, J. M., Dunn, N. R., Bellusci, S. and Hogan, B. L. (1999). Bmp signaling regulates proximal-distal differentiation of endoderm in mouse lung development. Development 126,4005 -4015.[Abstract]
Weaver, M., Dunn, N. R. and Hogan, B. L. (2000). Bmp4 and Fgf10 play opposing roles during lung bud morphogenesis. Development 127,2695 -2704.[Abstract]
Weaver, M., Batts, L. and Hogan, B. L. (2003). Tissue interactions pattern the mesenchyme of the embryonic mouse lung. Dev. Biol. 258,169 -184.[CrossRef][Medline]
Weidenfeld, J., Shu, W., Zhang, L., Millar, S. E. and Morrisey, E. E. (2002). The WNT7b promoter is regulated by TTF-1, GATA6, and Foxa2 in lung epithelium. J. Biol. Chem. 277,21061 -21070.[Abstract/Free Full Text]
White, A. C., Xu, J., Yin, Y., Smith, C., Schmid, G. and Ornitz, D. M. (2006). FGF9 and SHH signaling coordinate lung growth and development through regulation of distinct mesenchymal domains. Development 133,1507 -1517.[Abstract/Free Full Text]
White, A. C., Lavine, K. J. and Ornitz, D. M. (2007). FGF9 and SHH regulate mesenchymal Vegfa expression and development of the pulmonary capillary network. Development 134,3743 -3752.[Abstract/Free Full Text]
Ying, Q. L., Nichols, J., Chambers, I. and Smith, A. (2003). BMP induction of Id proteins suppresses differentiation and sustains embryonic stem cell self-renewal in collaboration with STAT3. Cell 115,281 -292.[CrossRef][Medline]
Yokota, Y., Mansouri, A., Mori, S., Sugawara, S., Adachi, S., Nishikawa, S. and Gruss, P. (1999). Development of peripheral lymphoid organs and natural killer cells depends on the helix-loop-helix inhibitor Id2. Nature 397,702 -706.[CrossRef][Medline]
Yokota, Y., Mori, S., Nishikawa, S. I., Mansouri, A., Gruss, P., Kusunoki, T., Katakai, T. and Shimizu, A. (2000). The helix-loop-helix inhibitor Id2 and cell differentiation control. Curr. Top. Microbiol. Immunol. 251, 35-41.[Medline]
Yokota, Y., Mori, S., Narumi, O. and Kitajima, K. (2001). In vivo function of a differentiation inhibitor, Id2. IUBMB Life 51,207 -214.[Medline]
Zhou, Q., Law, A. C., Rajagopal, J., Anderson, W. J., Gray, P. A. and Melton, D. A. (2007). A multipotent progenitor domain guides pancreatic organogenesis. Dev. Cell 13,103 -114.[CrossRef][Medline]

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