Pallister–Hall syndrome (PHS) is a rare disorder caused by mutations in GLI3 that produce a transcriptional repressor (GLI3R). Individuals with PHS present with a variably penetrant variety of urogenital system malformations, including renal aplasia or hypoplasia, hydroureter, hydronephrosis or a common urogenital sinus. The embryologic mechanisms controlled by GLI3R that result in these pathologic phenotypes are undefined. We demonstrate that germline expression of GLI3R causes renal hypoplasia, associated with decreased nephron number, and hydroureter and hydronephrosis, caused by blind-ending ureters. Mice with obligate GLI3R expression also displayed duplication of the ureters that was caused by aberrant common nephric duct patterning and ureteric stalk outgrowth. These developmental abnormalities are associated with suppressed Hedgehog signaling activity in the cloaca and adjacent vesicular mesenchyme. Mice with conditional expression of GLI3R were utilized to identify lineage-specific effects of GLI3R. In the ureteric bud, GLI3R expression decreased branching morphogenesis. In Six2-positive nephrogenic progenitors, GLI3R decreased progenitor cell proliferation reducing the number of nephrogenic precursor structures. Using mutant mice with Gli3R and Gli3 null alleles, we demonstrate that urogenital system patterning and development is controlled by the levels of GLI3R and not by an absence of full-length GLI3. We conclude that the urogenital system phenotypes observed in PHS are caused by GLI3R-dependent perturbations in nephric duct patterning, renal branching morphogenesis and nephrogenic progenitor self-renewal.
Pallister–Hall syndrome (PHS) (OMIM# 146510) is a rare autosomal dominant disorder characterized by hypothalamic harmatoma, polydactyly, imperforate anus and urogenital defects (1–7). PHS is caused by genetic mutations that alter the coding sequence of the middle-third of the transcription factor GLI3 (6). Mutations outside of this region cause a related but distinct disorder named Greigs cephalopolysyndactyly syndrome (GCPS) (OMIM# 175700) (8). Urogenital malformations in PHS include renal aplasia, renal hypoplasia, vesicoureteral reflux, hydroureter and a common urogenital opening. The frequency and penetrance of each of these abnormalities is variable but has not been precisely defined (2,3,8,9). GLI3 can act as a transcriptional activator or repressor and is dependent upon the state of Hedgehog (HH) signaling. Frameshift, insertional or point mutations found in PHS cases produce a peptide product that acts as an obligate transcriptional repressor (GLI3R) with varying degrees of activity and phenotypic severity (1–3,8). It is suggested that PHS is caused by increased GLI3-dependent transcriptional repression and not a lack of transcriptional activation that ultimately disrupts a domain of HH signaling during embryogenesis (1). In the context of urogenital system development, HH signaling and the effects of GLI3R are not well defined.
Mouse models have provided a basis for understanding the embryologic origins of PHS phenotypes and implicated HH signaling in the normal development of the kidney (10–14). Our lab has previously demonstrated that the loss of Shh, a ligand of the HH signaling pathway, causes renal agenesis or a single ectopic dysplastic kidney along the dorsal body wall (12). When Gli3 is genetically removed in a Shh−/− background, kidney induction is restored, suggesting that GLI3R controls ureteric induction (12). We have also demonstrated that ectopic activation of HH signaling disrupts ureteric branching morphogenesis by inhibiting RET–WNT11 signaling in a GLI3R-dependent fashion (15). Moreover, HH signaling activity in the periureteric mesenchyme is required for the differentiation of periureteric smooth muscle and urinary pacemaker cells that mediate urinary peristalsis (11,14,16). While these findings show that GLI3R is pathogenic in the context of altered upstream HH signaling effectors, the ligand-independent effects of GLI3R during kidney development have not been elucidated.
Here, we define a role for GLI3R in controlling kidney size through branching morphogenesis and nephrogenesis, and patterning of the urogenital sinus using mouse models of PHS [the Gli3Δ699 allele (10), and the conditional Rosa26Gli3TFLAG allele (17)]. Moreover, we demonstrate a domain of HH signaling in the nascent urogenital system that is disrupted by GLI3R. Finally, we demonstrate that urogenital system development in the context of PHS is dependent upon the levels of GLI3 repression and not a loss of GLI3 activation.
Obligate GLI3R expression causes a complex urogenital system phenotype
We investigated mechanisms by which GLI3R disrupts murine kidney development by initially analyzing the embryonic phenotype of Gli3Δ699/Δ699 mutant embryos at E18.5. All mutant embryos were characterized by marked hydroureter (Fig. 1A′ and A″), hydronephrosis (Fig. 1A′, A″, B′ and B″) and a thin renal cortex (Fig. 1B′ and B″). Two additional renal phenotypes were observed: (i) renal hypoplasia (n = 4/7, Fig. 1A′) and (ii) a bi-lobed kidney with a single ureter (n = 3/7, Fig. 1A″ and B″). In contrast, no abnormalities were observed in Gli3+/+ or Gli3Δ699/+ embryos (Fig. 1A and B). Collecting system dilatation was absent in Gli3Δ699/Δ699 embryos at E15.5, but confirmed the presence of hypoplastic renal tissue or a hypoplastic bi-lobed kidney (Fig. 1C′ and C″). Analysis of kidney volume and nephron number (performed by volumetric analysis of PAS-stained serial kidney sections and WT1 immunostaining) demonstrated a 53% decrease in volume (n = 11, P = 0.0074) and a 43% decrease in nephron number (n = 11, P<0.0001) in Gli3Δ699/Δ699 embryos compared with WT controls. Qualitative analysis of glomeruli, identified by WT1, demonstrated comparable morphology between mutant and control kidneys (data not shown). Together, these data demonstrate murine urogenital system phenotypes consistent with those observed in humans with PHS.
GLI3R impairs caudal nephric duct patterning and uretero-vesicular insertion
Next, we investigated the embryologic mechanisms underlying hydroureter in Gli3Δ699/Δ699 mice. Our published work using intrapelvic dye injections demonstrated continuity between the renal pelvis and ureter (14). Here, we analyzed the continuity between the ureter and the bladder in mice expressing both the Hoxb7-Cre and Rosa26lacZ reporter alleles (Hoxb7-Cre;Rosa26lacZ;Gli3Δ699/Δ699 referred to here as Gli3Δ699/ Δ699;UBlacZ) such that lacZ is expressed in the ureteric epithelium in a Cre-dependent manner. In controls at E16.5, ureters inserted bilaterally into the bladder at the trigone (Fig. 2A). In contrast, mutant mice demonstrated blind-ended ureters (Fig. 2A′, outlined in red) that failed to reach the bladder. Qualitative analysis of Gli3Δ699;UBlacZ urogenital ridges harvested at E12.5 revealed a shortened ureter that failed to maintain position with the caudal-most portion of the nephric duct at an embryological stage when the distal ureter is expected to be abutting the cloaca (Fig. 2B and B′, asterisk). In support of this observation, quantitation of the position of the ureteric stalk relative to the tip of the common nephric duct at E11.5 revealed that the distance between the ureteric bud site and the tip of the CND was 56.9% (P = 0.004) longer in mutants with no significant difference in overall nephric duct length. Moreover, nuclear fast-red staining of Gli3Δ699;UBlacZ histologic sections at E10.5 demonstrated abnormal CND morphology in mutant mice (Fig. 2C–D′, arrowheads). Together, these data demonstrate that GLI3R antagonizes caudal positioning of the ureteric bud site along the nephric duct consistent with a ureteric insertional defect in the bladder.
GLI3R inhibits ureteric bud outgrowth
The appearance of a bi-lobed kidney in a subset of Gli3Δ699/Δ699 mutant mice suggested a possible abnormality of ureteric budding that produced a double collecting system. We investigated this possibility in E11.5 Gli3Δ699/Δ699 embryos carrying the Hoxb7-Cre and Rosa26lacZ alleles. Whole-mount imaging of the urogenital ridge in Hoxb7-Cre;Rosa26lacZ/+;Gli3Δ699/Δ699 mice demonstrated a thin and short ureteric stalk with relatively normal looking ureteric tips (Fig. 2E′). Further, a ‘Y’-shaped collecting system was observed unilaterally in four of six urogenital ridges imaged (Fig. 2E′). To define the morphologic events that give rise to this Y-shaped collecting system, ureteric budding was analyzed in Gli3Δ699/Δ699 mice in which expression of Rosa26tdTomato was controlled by Hoxb7-Cre. Ureteric outgrowth was imaged in urogenital cultures established at E10.5 using real-time fluorescent microscopy. Nephric ducts were live imaged every 5 min over a 48 h period. In Hoxb7-Cre;Rosa26tdTomato/+;Gli3+/+ control mice, the nascent ureteric bud was located caudally, elongated and the elongated ureteric stalk bifurcated into a T-shaped structure (Fig. 3A–D, Supplementary Material, Movie S1). In contrast, in Hoxb7-Cre;Rosa26tdTomato/+;Gli3Δ699/Δ699 mice, the nascent ureteric bud outgrowth appeared misshapen, had no caudal bias and was slow growing (Fig. 3A′–D′, Supplementary Material, Movie S2). Surprisingly, in mutant mice, the ureteric bud tips began to branch to form a T-shaped structure before the ureteric stalk had sufficiently elongated (Fig. 3C′). The resulting tips invaded the metanephric mesenchyme at an angle causing a Y-shaped collecting system rather than a ‘T’ shape (Fig. 3D′). The resulting branch generation remained extra-metanephric giving the appearance of two collecting systems that ultimately converge into one ureteric stalk consistent with the double collecting system phenotype observed in later-staged embryos.
To investigate mechanisms that could explain abnormal ureteric induction in Gli3Δ699/Δ699 mice, we analyzed cell proliferation, apoptosis and gene expression. The proliferative index of ureteric bud cells, assessed by immunofluorescence for pHH3 and cytokeratin using midsagittal tissue sections generated at E11.5, did not differ between mutant and control mice (n = 7, data not shown). Moreover there was no evidence of ureteric apoptosis as indicated by activated caspase-3 staining (n = 7). Since it has been suggested that a pre-inductive burst of cell proliferation in the nephric duct determines the complement of cells that comprise the ureteric bud (18), we analyzed cell proliferation in this domain at E10.5 using pHH3 and E-cadherin-stained sections. Our results indicate that the proliferative index in the ND at the ureteric bud site was not significantly different between Gli3Δ699/Δ699 and control mice (n = 5, P = 0.1469).
To investigate the possible effect of GLI3R expression on the signaling network required for ureteric bud induction and outgrowth, we analyzed expression of Gdnf, Ret, Wnt11 and their downstream transcriptional targets by whole-mount in situ hybridization (Supplementary Material, Fig. S1A–E′). Considering the difference in metanephric size, the expression of Gdnf, Ret, Wnt11, Etv4 and Etv5 was not significantly altered in Gli3Δ699/Δ699 mice at E11.5. Further, lack of perturbation in the expression of Osr1 confirmed that GLI3R does not alter the size of the metanephric domain (Supplementary Material, Fig. S1F and F′). Together, these data suggest that GLI3R controls ureteric bud induction and outgrowth via mechanisms independent of cell number control and the Gdnf–Ret–Wnt11 axis.
GLI3R suppresses an embryonic caudal domain of HH signaling
To assess the state of HH signaling activity that could contribute to the nephric duct patterning defects observed in the Gli3Δ699 model, the Ptc1lacZ allele was crossed into the Gli3Δ699 genetic background to generate Gli3Δ699/Δ699;Ptc1lacZ/+ and Gli3+/+;Ptc1lacZ/+ embryos. Here, the state of HH signaling is indicated by Ptc1lacZ activity. Transverse lacZ-stained tissue sections, generated from E11.5 embryos, demonstrated the domain of HH signaling (Fig. 4A and B). LacZ expression was observed in the gut tube (Fig. 4A and A′, asterisk) that lies along the ventral midline as well as the notochord and adjacent mesenchyme along the dorsum of the embryo (Fig. 4A and A′, arrowhead) in both Gli3Δ699/Δ699;Ptc1lacZ/+ and Gli3+/+;Ptc1lacZ/+ embryos. However, the intensity of lacZ expression was reduced in Gli3Δ699/Δ699;Ptc1lacZ/+ embryos, indicating that HH signaling is attenuated (Fig. 4A and A′). Notably, HH signaling activity was not detected in the nephric duct (Fig. 4C and C′, arrowhead) or nascent ureteric bud (Fig. 4D and D′, arrowhead) in Gli3Δ699/Δ699;Ptc1lacZ/+ and Gli3+/+;Ptc1lacZ/+ embryos suggesting that these structures are naturally devoid of HH signaling activity at this embryonic stage. In more caudal transverse sections (Fig. 4B and B′) that spanned the common nephric duct, cloaca and vesicular mesenchyme, robust HH signaling activity was detected in Gli3+/+;Ptc1lacZ/+ embryos. In contrast, HH signaling activity was markedly reduced in this domain in Gli3Δ699/Δ699;Ptc1lacZ/+ embryos (Fig. 4E′ and F′). Together, these results identify the midline metanephric mesenchyme, common nephric duct, cloaca and vesicular mesenchyme as HH signaling domains that are disrupted by obligate GLI3R expression.
GLI3R acts autonomously in the ureteric cell lineage to decrease renal branching morphogenesis
Gli3Δ699/Δ699mice are characterized by renal hypoplasia and decreased nephron number. Nephron number is determined, in part, by the number of ureteric branches generated during the process of branching morphogenesis (19). Accordingly, we analyzed the effect of GLI3R on this process in a cell-lineage-specific manner. Mice carrying the UB-specific Hoxb7-Cre allele or the nephrogenic mesenchyme-specific Six2-Cre allele were bred with mice containing the Rosa26Gli3TFLAG allele (Cre-dependent expression of GLI3R from the ubiquitously expressed Rosa26 locus) to generate Hoxb7-Cre;Rosa26Gli3TFLAG/+ (UBGLI3R) or Six2-Cre;Rosa26Gli3TFLAG/+ (NMGLI3R) embryos. Ureteric branch number was quantified in tissue isolated at E12.5 from Gli3Δ699/Δ699 (Fig. 5B), UBGLI3R (Fig. 5C) and NMGLI3R (Fig. 5E) mice. Branching was decreased by 51% (n = 8, P > 0.0001) in Gli3Δ699/Δ699 kidneys and 47% (n = 7, P = 0.0002) in UBGLI3R kidneys (Fig. 5F). In contrast, no decrease was detected in NMGLI3R mutants (n = 4, P = 0.125, Fig. 5E). A single allele of Gli3Δ699 in UBGLI3R mutants did not further decrease branching morphogenesis (Fig. 5D). Taken together, these data demonstrate that GLI3R in the ureteric cell lineage inhibits renal branching morphogenesis.
GLI3R acts autonomously in the metanephric mesenchyme to control nephron number
Since GLI3R is expressed in all renal cell types in Gli3Δ699/Δ699 kidneys, it is possible that reduced branching morphogenesis does not fully explain the deleterious effects of GLI3R on nephron number. Thus, we investigated whether GLI3R affects the process of nephrogenesis after the point of metanephric induction by ureteric bud tips. Nephrogenesis was examined in Gli3Δ699/Δ699 kidneys using immunostained tissue sections. At E15.5, all intermediate nephrogenic structures (vesicles, comma- and S-shaped) were equally reduced by 48 ± 5% in Gli3Δ699/Δ699 kidneys (Fig. 6F). Next, we determined if GLI3R acts directly in the metanephric mesenchyme to control nephrogenesis and nephron number. GLI3R was conditionally expressed using the nephrogenic mesenchyme-specific Six2-Cre allele (Six2-Cre;Rosa26Gli3TFLAG/+, referred to as NMGLI3R). At E15.5, NMGLI3R kidneys were hypoplastic (Fig. 6A and A′). Cells expressing GLI3R, marked using an anti-FLAG antibody, constituted 49.4 and 89.8% of the SIX2-positive population at E13.5 and E15.5, respectively (Fig. 6B and C). At E15.5, the number of SIX2-positive cells was decreased and the distribution of cells was irregular and discontinuous in NMGLI3R mutants (Fig. 6C). Since nephrogenesis is dependent on Six2-positive cell self-renewal, we measured SIX2-positive cell proliferation using anti-pHH3 and anti-SIX2 (Fig. 6D and D′). At E15.5, the proliferative index was reduced by 69.4% (n = 10, P = 0.0042, Fig. 6E). There was no evidence of apoptosis as indicated by activated caspase-3 staining (data not shown). These data indicate that obligate GLI3R in the nephrogenic mesenchyme inhibits nephrogenic mesenchyme self-renewal. Despite the decrease in SIX2-positive cell number, FLAG-positive cells were found in all nephrogenic structures and mature glomeruli (Fig. 6C, arrowheads), demonstrating that GLI3R-expressing cells can contribute to all stages of nephrogenesis. Further, consistent with the observed equivalent decrease in nephrogenic structures in Gli3Δ699/Δ699 mice, intermediate nephrogenic structures were also decreased in NMGLI3R mice (reduction in number: renal vesicles, 74.8%; comma-shaped bodies, 76.0%; S-shaped bodies, 81.2%). Together, these data show that GLI3R acts within Six2-positive nephrogenic progenitors to decrease their number but does arrest the process of nephrogenesis.
Kidney development is disrupted by GLI3 repressor and not a loss of GLI3 activator
The disruption in GLI3 in PHS generates a GLI3R and, thus, limits expression of full-length GLI3 which acts as a transcriptional activator. We determined whether the renal phenotypes observed in Gli3Δ699/Δ699 mutants are due to the presence of increased levels of GLI3R or to a loss of full-length GLI3. Gli3Δ699/xtJ embryos were generated and kidneys were harvested at E18.5. Here, the dose of GLI3R is allelically reduced in the absence of transcriptionally active GLI3. Strikingly, Gli3Δ699/xtJ mutant kidneys were phenotypically normal in comparison to Gli3+/+ and Gli3Δ699/+ controls (Fig. 7A–D). These data provide compelling evidence that kidney development is sensitive to the levels of GLI3R and not to those of full-length GLI3.
Development of the permanent mammalian kidney is a complex and highly integrated process that occurs between multiple cell lineages and involves ureteric induction, renal branching morphogenesis and nephrogenesis. Our lab has previously identified a requirement for HH-GLI signaling during kidney induction that is dependent upon levels of the transcriptional repressor GLI3R (12). Despite this implication, the GLI3-dependent cellular and lineage-specific mechanisms that give rise to the variety of urinary tract-associated phenotypes in PHS remained unclear.
Detailed study of the Gli3Δ699 mouse model and accompanying lineage-specific GLI3R expression models, described here demonstrate that obligate GLI3R impairs ureteric induction and renal branching morphogenesis by impeding ureteric stalk outgrowth (Fig. 8A and A′). Delayed ureteric stalk outgrowth results in renal hypoplasia, duplication of the renal collecting system and hydroureter and hydronephrosis. Reduced branching morphogenesis is specifically caused by GLI3R in the ureteric epithelium at E11.5 and onward leading to a marked reduction in ureteric tip number (Fig. 8C and C′). Canonical branching signaling pathways remain intact at the onset of reduced ureteric branching, suggesting that GLI3R controls a novel and unique subset of genes required for branching morphogenesis. Given the spatial differences in HH signaling within the kidney, it is likely that GLI3R specifies genetic programs unique to the ureteric tip domain at the expense of the ureteric stalk domain. If this is true, then a differential analysis of the genetic profile found in ureteric tip cells and ureteric stalk cells is likely to reveal GLI3R-dependent signaling cascades.
Nephron formation is a complex and highly integrated process that depends on multiple signaling events across a number of distinct pathways. Nephrons derive from the nephrogenic mesenchyme as a pool of self-renewing multipotent cells that are dependent on SIX2 expression. The data presented here demonstrate that GLI3R controls nephrogenic mesenchyme self-renewal in a Six2-independent manner (Fig. 8B and B′). It remains unclear if GLI3R acts in parallel with or downstream of Six2 to control this self-renewal process. Although the renal cortex does not have an active HH signaling domain, these data demonstrate that the nephrogenic mesenchyme is indeed sensitive to increased levels of GLI3R.
The severity of GLI3 mutations found in PHS patients is believed to be associated with the severity of disease phenotype (2,3). Here we demonstrate, using germline mouse models, that urogenital system development is sensitive to the levels of GLI3R but not to full-length GLI3 in contrast to limb development that is impaired by a loss of full-length GLI3 (20). Interestingly, genetic reduction in the mouse Gli3Δ699 allele to hemizygosity restores kidney development. Recent evidence suggested that the terminal amino-acid sequence produced by the Gli3Δ699 allele reduces the potency of the peptide product (21). This observation may explain the autosomal recessive nature of the Gli3Δ699 PHS model presented here. Serendipitously, the reduced potency of the Gli3Δ699 allele has facilitated a more detailed analysis of the specific processes disrupted by obligate GLI3R in the developing kidney. Expression of the Rosa26Gli3TFLAG allele, used here to investigate the cell-lineage-specific effects of GLI3R, generated phenotypes in the ureteric and nephrogenic lineages. Since the relative potency of the Rosa26Gli3TFLAG allele compared with PHS mutations is unknown, it remains unclear whether the severity of the phenotypes observed in lineage-specific Rosa26Gli3TFLAG models phenocopies many of the renal–urinary pathologies in PHS.
Urogenital system malformations have been reported in PHS cases and are marked by hydroureter, hydronephrosis and a common urogenital opening (2,3,6). Consistent with these findings, our data demonstrate that GLI3R disrupts caudal nephric duct patterning by altering the ureteric bud site relative to the distal tip of the nephric duct. Our data also illustrate a previously undefined HH signaling domain at E11.5 in the caudal nephric duct and adjacent mesenchyme that is sensitive to the levels of GLI3R. Indeed, other more distal elements of the urinary tract including the bladder are sensitive to HH signaling levels during embryogenesis (22,23). When HH signaling is abrogated by a temporal deletion of Shh, a population of peri-cloacal mesenchyme is lost that leads to hydroureter and hydronephrosis (22). Known HH responsive effectors of bladder development include genes responsible for smooth muscle differentiation (16,23,24). Connectivity between the CND and bladder is established in part by the transcription factor Gata3 in an RET-dependent fashion (25). We have shown that Ret expression in a germline model of PHS is unperturbed, suggesting that HH signaling may act via a novel mechanism to control CND patterning and vesicular insertion. It remains unclear whether the CND is competent in a germline model of PHS to establish continuity with the cloaca or whether there is a defect inherent to the cloaca that inhibits CND invasion.
Our findings demonstrate the contributions of GLI3R to the developing renal–urinary system in germline and lineage-specific models of PHS. We conclude that GLI3R alters the normal HH signaling domain in the caudal embryo, and that GLI3R impairs nephric duct patterning, renal branching morphogenesis and nephrogenic mesenchyme self-renewal. Whereby some non-renal features of PHS are caused by a loss of full-length GLI3, we conclude that urogenital system development in PHS is dependent on increased levels of GLI3R. Our findings provide novel insight into the embryological origins of the pathologies found in renal–urogenital systems in PHS.
Materials and Methods
The Gli3Δ699 mouse line was previously described (10) and maintained on a mixed C57Bl6 background. The Hoxb7-Cre (26) (UB) and Six2-Cre (27) (NM) mouse lines were previously described and maintained on a mixed background. The Rosa26Gli3TFLAG allele was previously described, and homozygotes were maintained on an inbred C57Bl6 background. The Rosa26lacZ allele was previously described, and homozygotes were maintained on an outbred CD1 background. The Rosa26tdTomato allele was previously described, and homozygotes were maintained on an inbred C57Bl6 background. All animals were used in accordance with our animal use protocol at the Toronto Centre for Phenogenomics and in compliance with the Canadian Council on Animal Care.
E10.5 urogenital ridges were resected in DMEM:F12 + 1% PenStrep (Invitrogen), bisected along the sagittal midline and transferred to 3 μm transwell filter inserts. Ridges were cultured using DMEM:F12 (Invitrogen) + 10% FBS (Gibco) + 1% PenStrep (Invitrogen) for 48 h and imaged every 5 min. Cultures were kept humidified at 37°C in a 5% CO2 atmosphere with a Pecon XL chamber and Zeiss incubation module fitted to an Axiovert 200 M inverted epifluorescent microscope using AxioVision 4.8 software (Zeiss Canada).
Tissue preparation and histology
Tissue harvested for histology, section immunofluorescence and section in situ hybridization was fixed in 4% PFA: PBS overnight at 4°C and dehydrated in 70% ethanol to be processed for paraffin embedding. E10.5 and E11.5 tissue was first embedded in Histogel (Thermo Fisher) to orient the specimen and then subsequently dehydrated and processed for paraffin embedding. Tissue harvested for whole-mount immunofluorescence was fixed using −20°C 4:1 (Methanol:DMSO) Dent's Fix and stored at −20°C until use. Whole tissue harvested for lacZ staining was fixed and washed as previously described and stained for 48 h at 37°C. LacZ-stained tissue was subsequently processed for paraffin embedding and sections were counterstained using nuclear fast red.
Section immunofluorescence was performed on 4 μm paraffin sections as previously described; however, Dako serum-free protein block was used for blocking, primary and secondary incubation buffers. Whole-mount immunofluorescence was performed as previously described. The following antibodies were used: α-Calbindin-D28K (1:100) (Sigma, C9848 and C7354), α-activated Caspase 3 (1:500) (Cell Signaling, 5A1E), α-Cited 1 (1:150) (NeoMarkers, RB-9219-P0), α-pan Cytokeratin (1:100) (Sigma, C2562), α-E-cadherin (1:250) (Cell Signaling, 24E10), α-GFP (1:250) (Rockland, 600–401–215), α-Gli3 (Sigma, 2C9), α-NCAM (1:250) (Sigma, C9672), α-phospho-Histone H3 (1:250) (Cell Signaling, D2C8 & 6G3), α-Sall1 (1:250) (Abcam, ab31526), α-Six2 (1:250) (Proteintech, 11562-1-AP), α-SMA (1:250) (Sigma, A5228), α-RFP (1:250) (Rockland, 600-401-379), α-WT1 (1:250) (Dako, Clone 6F-H2).
RNA in situ hybridization
Section and whole-mount RNA in situ hybridization was performed as previously described. DIG-labeled riboprobes were made as previously described from PCR linearized plasmid DNA. The following probes were newly generated and sequence verified from E15.5 mouse kidney cDNA (CD-1 background): Bmp4, Raldh2, Etv4, Etv5.
This work was supported by a Canadian Institutes of Health Research Canada Graduate Scholarship Award (to J.B.) and by grants from the Canadian Institutes of Health Research and Canada Research Chairs Program (to N.D.R.).
We thank Ulrich Ruther for the Gli3Δ699/+mice, Carlton Bates for the Hoxb7-Cre mice and Chi-chung Hui for the Ptc1lacZ/+ mice.
Conflict of Interest statement. None declared.