Edar is a downstream target of beta-catenin and drives collagen accumulation in the mouse prostate

ABSTRACT Beta-catenin (CTNNB1) directs ectodermal appendage spacing by activating ectodysplasin A receptor (EDAR) transcription, but whether CTNNB1 acts by a similar mechanism in the prostate, an endoderm-derived tissue, is unclear. Here we examined the expression, function, and CTNNB1 dependence of the EDAR pathway during prostate development. In situ hybridization studies reveal EDAR pathway components including Wnt10b in the developing prostate and localize these factors to prostatic bud epithelium where CTNNB1 target genes are co-expressed. We used a genetic approach to ectopically activate CTNNB1 in developing mouse prostate and observed focal increases in Edar and Wnt10b mRNAs. We also used a genetic approach to test the prostatic consequences of activating or inhibiting Edar expression. Edar overexpression does not visibly alter prostatic bud formation or branching morphogenesis, and Edar expression is not necessary for either of these events. However, Edar overexpression is associated with an abnormally thick and collagen-rich stroma in adult mouse prostates. These results support CTNNB1 as a transcriptional activator of Edar and Wnt10b in the developing prostate and demonstrate Edar is not only important for ectodermal appendage patterning but also influences collagen organization in adult prostates. This article has an associated First Person interview with the first author of the paper.


INTRODUCTION
The mouse prostate derives from the urogenital sinus (UGS), a fetal structure at the base of the bladder consisting of endodermderived epithelium, mesoderm-derived mesenchyme and other cell types. Prostate development is initiated by androgen-induced signals from UGS mesenchyme (Cunha and Lung, 1978;Goldstein and Wilson, 1975;Lasnitzki and Mizuno, 1980). Prostate ductal progenitors ( prostatic buds) arise as solid epithelial projections in a periodic pattern to establish position and number of mature prostatic ducts.
The Wingless/beta-catenin (Wnt/CTNNB1) is an androgen sensitive signaling pathway critical for prostatic bud formation (He et al., 2018). CTNNB1 and its target genes are present in prostatic buds from the earliest stage of prostate development and continuing at least through postnatal branching morphogenesis (Francis et al., 2013;Simons et al., 2012). Chemical inhibition or genetic deletion of CTNNB1 in UGS epithelium completely prevents prostatic bud formation (Mehta et al., 2013;Simons et al., 2012), while excessive CTNNB1 activation by genetic gain-offunction increases the inter-bud interval and reduces the quantity of prostatic buds formed (Mehta et al., 2013). How CTNNB1 is activated during prostate development and how its activity is restricted to prostatic bud tips is not fully understood.
Co-localization of CTNNB1 target genes with Edar and Wnt10b in prostatic bud tips (Keil et al., 2012a;Mehta et al., 2011) led us to hypothesize that EDAR is induced by CTNNB1 in the developing prostate and patterns prostatic buds by controlling CTNNB1 domain size as it does in ectoderm-derived appendages. Here, we reveal that Eda, Edar and Wnt10b are expressed during prostatic bud formation, elongation and branching morphogenesis. We demonstrate that ectopic CTNNB1 expression induces Edar and Wnt10b in UGS epithelium. We use genetic approaches to show that Edar is expendable for in vivo prostatic bud patterning. Genetically increasing or decreasing expression of Edar has no discernable influence on prostatic bud development. However, genetic gain-offunction experiments demonstrate that EDAR overexpression affects prostate stromal composition by resulting in an abnormally thickened fibromuscular stroma containing excessive collagen. This is the first study to demonstrate EDAR and CTNNB1 signaling pathways intersect during formation of an endoderm-derived tissue (prostate) and EDAR activity influences prostatic extracellular matrix organization.

RESULTS
Edar mRNA localizes to prostatic epithelium during bud formation and branching morphogenesis (Keil et al., 2012a). To determine whether other pathway components are expressed, in situ hybridization (ISH) was used to visualize the EDAR ligand Eda and the putative downstream target of EDAR signaling (Wnt10b) during the periods coinciding with bud elongation (18 days post conception, dpc) and branching morphogenesis ( postnatal day 5, P5). Eda mRNA is present in superficial urethral epithelium at 18 dpc and P5. Edar is expressed exclusively in prostate bud tips at 18 dpc, but found much more diffusely in the stroma at P5. Wnt10b is found only in prostatic bud distal tips at both 18 dpc and P5 (Fig. 1). Together, these results indicate that key EDAR signaling pathway components are present at the appropriate time and space to participate in prostatic ductal development.
CTNNB1 drives expression of Edar and its downstream target Wnt10b (Zhang et al., 2009). To test whether CTNNB1 activates Edar and Wnt10b in developing prostate, we generated mice expressing activated the dominant stable Ctnnb1 tm1Mmt gain-offunction (GOF) allele using Shh creERT2 to generate Ctnnb1 iGOF mice. The mice harbor a floxed Ctnnb1 exon 3, which, when subjected to CRE-mediated recombination, encodes a functional and highly stable CTNNB1 protein form that accumulates in cells. Cre activity was activated by tamoxifen administration to the dam on 13 and 14 dpc. We showed previously that this tamoxifen dosing strategy does not in itself interfere with prostatic bud formation and that in this particular mouse strain, CTNNB1 accumulates in discrete cell islands readily discernable in tissue sections (Mehta et al., 2013). EDAR signaling pathway mRNAs were assessed at 18 dpc, after completion of prostatic budding in control mice. The Edar and Wnt10b mRNAs are noticeably more abundant in Ctnnb1 iGOF mutant urethras compared to controls and localize to cell islands ( Fig. 2) where we localized CTNNB1 overexpression (Mehta et al., 2013). Eda mRNA is not detected within these cell islands and is noticeably less abundant in Ctnnb1 iGOF mice compared to controls (Fig. 2). These results are consistent with CTNNB1 driving the expression of Edar and Wnt10b in the developing prostate.
CTNNB1 is required for prostatic bud formation (Mehta et al., 2013). To test whether Edar is required for the downstream activities of CTNNB1, we used a genetic approach involving Edar loss-of-function (LOF) mice that carry a missense mutation (Headon and Overbeek, 1999), and Edar transgenic GOF mice that overexpress Edar in the same cells where it is normally expressed (Mou et al., 2008). P1 male mouse lower urinary tracts were collected from each strain and stained in wholemount to visualize Nkx3-1 marked prostatic buds. There are no appreciable strainrelated differences in prostate bud size, organization, or number (Fig. 3). These results indicate that Edar is not required for prostatic bud formation, is not sufficient to induce changes in prostatic bud formation, and that CTNNB1 acts through an Edar-independent mechanism to control prostatic bud formation.
To identify potential roles for CTNNB1 and EDAR signaling in prostate maturation, we next examined adult prostates from control, Edar GOF , and Edar LOF mice. Prostates from these mice were examined at P50, after sexual maturation is complete. No gross abnormalities were observed in either mouse strain. All prostate lobes were present and appeared normal in location, size and morphology. Histological analysis revealed that prostate ducts from all groups are lined by a continuous luminal epithelial cell layer bounded by a basal epithelial cell layer (Fig. 4), evidence that prostate epithelial cell organization is grossly normal in Edar GOF and Edar LOF mice. However, Edar GOF mouse prostates exhibit an abnormally thickened and eosinophilic periductal stroma, indicative of high collagen content (Fig. 4).
We next evaluated collagen composition in adult male Edar GOF mutant mice. CTNNB1/Wnt signaling regulates extracellular matrix density in other organs including skin (Beyer et al., 2012;Lam and Gottardi, 2011;Wei et al., 2011), but how prostatic collagen is deposited and organized during prostate maturation has not been previously examined. Studies aimed at understanding prostate matrix regulation could reveal valuable insights into fibrotic prostatic disease, which has been associated with voiding dysfunction in adult men (Cantiello et al., 2013;Gharaee-Kermani et al., 2013;Ma et al., 2012). To visualize the prostatic collagen network, we used Picrosirius Red staining and fluorescent confocal microscopy in 5 μm tissue sections of Edar GOF and paired wild-type controls of the same mouse strain. Automated fiber detection software (CT-FIRE) was used to measure individual collagen fiber metrics including density, orientation, alignment, diameter and length. Collagen architecture in Edar GOF prostates is significantly denser and more fibrous than in controls (Fig. 5).

DISCUSSION
We found that CTNNB1 drives Edar expression in developing prostatic bud epithelium. CTNNB1 and EDAR were previously linked to ectodermal appendage development but this study links them in endodermal tissue development and sheds new light on our previous observation that CTNNB1-responsive target genes (Lef1, Axin2 and Wif1) colocalize with Edar and Wnt10b mRNAs in elongating prostatic bud tips (Keil et al., 2012a, b;Mehta et al., 2011). It is not known whether EDAR is expressed in the terminal portion of buds from other endoderm-derived tissues, such as lung, or whether EDAR refines CTNNB1 signaling in these organs as it does in ectodermal appendages.
CTNNB1-dependent EDAR activation establishes size and periodicity of ectodermal appendages (Drew et al., 2007;Zhang et al., 2009). Though prostatic bud patterning also requires CTNNB1 (Francis et al., 2013;Mehta et al., 2013;Simons et al., 2012), we showed here that this process does not require EDAR. Mouse prostatic buds form in the normal quantity and size when Edar is genetically ablated and when Edar is overexpressed within its normal expression domain.
Edar LOF and GOF mutations do not appreciably affect prostate epithelial maturation but do impact prostatic stromal matrix organization in adult males. In control adult males, the interductal space is largely devoid of thick collagen bundles, with a majority of the collagen residing in the fibromuscular tunica around ducts, but adult Edar GOF mutant mouse prostates inappropriately accumulate collagen fibers. Given the timing of these changes, we conclude that EDAR is not necessary for early prostate formation but is needed for long term prostatic collagen homeostasis. How EDAR regulates prostatic collagens is still unclear. It is possible that EDAR signaling during prostatic development expands progenitors giving rise to collagen producing cells. Alternatively, indirect epithelial EDAR signaling during sexual maturation may drive stromal collagen deposition or reduce stromal collagen degradation. Prostatic matrix composition has drawn considerable clinical interest in recent years for its potential involvement in mediating lower urinary tract symptoms. Prostatic collagen density associates with lower urinary tract symptoms in aging men (Cantiello et al., 2013;Cantiello et al., 2014;Ma et al., 2012). While inflammatory mediators and metabolic syndrome are defined mediators of prostatic fibrosis Gharaee-Kermani et al., 2013;Wong et al., 2014), the role of other factors, including genetic factors, has not been examined. Our results provide the first evidence that excessive EDAR signaling during prostatic development can lead to an abnormally dense collagen matrix within the prostate and emphasizes the need to examine new pathways as potential therapeutic targets for prostate disease.

In situ hybridization
Detailed protocols are available at the GUDMAP database, www.gudmap. org and were described previously . Primer sequences for generating PCR-amplified probe templates are listed in Table S1. The staining pattern for each hybridized riboprobe was assessed in at least three litter-independent mice per genotype. Control and mutant tissues were processed together in the same tubes and as a single experimental unit to allow for qualitative comparisons among biological replicates and between genotypes or treatment groups.

Hematoxylin and Eosin (H&E)
Adult prostate tissues were fixed in 4% paraformaldehyde, dehydrated in ethanol, cleared in xylene, infiltrated with paraffin and 5 µm sections were stained with Hematoxylin and Eosin. Brightfield imaging was performed using a Nikon E600 microscope (Nikon; Tokyo, Japan) using a 10× dry objective.

Picrosirius Red (PSR)
Adult prostate tissues were fixed in 4% paraformaldehyde, dehydrated in alcohol, cleared in xylene, infiltrated with paraffin, and three non-serial 5 µm sections were taken from three litter-independent mice per group. Sections were taken from approximate equivalent tissue depth and stained with PSR as described previously (Wegner et al., 2017). Fluorescent imaging was performed using a SP8 Confocal Microscope (Leica; Wetzlar, Germany) using a 20× oil immersion objective (HC PL Apo CS2 NA=0.75; Leica). Samples were excited using a 561 nm laser and emission was detected between 635 and 685 nm. Laser intensity and gain were held constant between images. Images were captured at 1024×1024 resolution using LAS X software (Leica; Wetzlar, Germany). Tile scanning was used to stitch together images and generate an image across the entire prostate section. Total collagen density was determined by measuring the area of PSR stain in each section compared to the total cross-sectional area of the section. Automated fiber detection software (CT-FIRE) was used to measure individual collagen fiber metrics including density, orientation, alignment, diameter, and length. CT-FIRE is publicly available from the University of Wisconsin Laboratory for Optical and Computational Instrumentation.

Statistics
For ISH experiments, experimental groups consisted of three to five UGSs from at least three independent litters. Images are representative of each treatment group. For PSR experiments, three non-serial dorsal prostate sections were imaged from three mice originating from three independent litters. A Levene's test was performed to test whether homogeneity of Fig. 3. EDAR is not required for prostatic bud formation and excessive EDAR does not change the number of prostatic buds formed. Lower urinary tracts from P1 male (A) control, (B) Edar transgenic gainof-function (Edar GOF ), and (C) Edar transgenic loss-of-function (Edar LOF ) mice were stained by ISH to visualize Nkx3-1 ( purple). Results are representative of three males per group. bl, bladder; sv, seminal vesicle. Arrowheads indicate prostatic buds. Scale bar: 500 µm. Fig. 4. Excessive EDAR causes increased periductal stromal thickness. Mouse prostate tissue sections (5 µm) were generated from male control (A) or transgenic Edar GOF (B) or Edar LOF (C) mice. Sections were stained with Hematoxylin and Eosin and imaged using bright field microscopy. Edar GOF appear to have increased in the periductal, eosinophilic stromal layer. Arrowheads mark areas of altered periductal stroma thickness. Scale bar: 100 µm.