edn1 and hand2 Interact in Early Regulation of Pharyngeal Arch Outgrowth during Zebrafish Development

Mark M. Sasaki; James T. Nichols; Charles B. Kimmel

doi:10.1371/journal.pone.0067522

Abstract

Endothelin-1 (Edn1) signaling provides a critical input to development of the embryonic pharygneal arches and their skeletal derivatives, particularly the articulating joints and the ventral skeleton including the lower jaw. Previous work in zebrafish has mostly focused on the role of Edn1 in dorsal-ventral (DV) patterning, but Edn1 signaling must also regulate tissue size, for with severe loss of the pathway the ventral skeleton is not only mispatterned, but is also prominently hypoplastic – reduced in size. Here we use mutational analyses to show that in the early pharyngeal arches, ventral-specific edn1-mediated proliferation of neural crest derived cells is required for DV expansion and outgrowth, and that this positive regulation is counterbalanced by a negative one exerted through a pivotal, ventrally expressed Edn1-target gene, hand2. We also describe a new morphogenetic cell movement in the ventral first arch, sweeping cells anterior in the arch to the region where the lower jaw forms. This movement is negatively regulated by hand2 in an apparently edn1-independent fashion. These findings point to complexity of regulation by edn1 and hand2 at the earliest stages of pharyngeal arch development, in which control of growth and morphogenesis can be genetically separated.

Citation: Sasaki MM, Nichols JT, Kimmel CB (2013) edn1 and hand2 Interact in Early Regulation of Pharyngeal Arch Outgrowth during Zebrafish Development. PLoS ONE 8(6): e67522. https://doi.org/10.1371/journal.pone.0067522

Editor: Yann Gibert, Deakin School of Medicine, Australia

Received: March 21, 2013; Accepted: May 20, 2013; Published: June 24, 2013

Copyright: © 2013 Sasaki et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

Funding: This research was supported by National Institutes of Health (NIH) RO1 DE13834 and PO1HD22486, and a NIH postdoctoral fellowships F32-086027 (to JTN) and F32-DE019056 (to MMS). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.

Competing interests: The authors have declared that no competing interests exist.

Introduction

Beginning with mutations isolated in the early large-scale genetic screens in zebrafish [1], [2] a large amount of information has accumulated on the genetic regulation of development of the pharyngeal arches of this species, and the region of the larval skeleton derived from the embryonic arches. Most of the studies focus on patterning of the first two arches, mandibular and hyoid, which by four days postfertilization (dpf), a day after hatching, have both developed cartilaginous elements with articulating joints between them. These elements in the first arch comprise the skeleton of the upper and lower larval jaws, and in the second the supports for the jaws, the buccal cavity, and the operculum that covers the gill chamber. The characterization of zebrafish mutants exhibiting prominent ventral cartilage and joint region defects in the anterior arches [2] complemented earlier work in mouse in identifying the Endothelin1 (Edn1) signaling pathway as being critical for arch patterning [3]. Edn1 secreted by ventral epithelial and arch mesoderm may function in the manner of a morphogen [4], part of the mechanism specifying dorsal-ventral (DV) identity in the neural crest-derived skeletal ectomesenchyme. Edn1-dependent specification includes dynamic and position-dependent upregulation in the responding cells of target genes encoding transcription factors. These include hand2, with expression restricted to the ventral patterning domain that forms the ventral cartilage elements, and a set of Dlx genes restricted more dorsally to the intermediate domain from which the joints and joint-related skeleton develops [5], [6], [7], [8], [9], [10], [11]. Proper patterning requires cross-talk among the Edn1-target genes. For example hand2 negatively regulates Dlx genes, serving as part of the regulation restricting the Dlx genes from more ventral expression [10], [12], [13].

Other recent work in zebrafish has identified additional signaling pathways, Notch and BMP, that interact with Edn1, and these studies fill in gaps in our understanding of arch patterning coming from just Edn1 signaling in isolation [14], [15], [16]. However, apart from arch patterning, the Edn1 signaling pathway must also play a critical role in the regulation of arch and pharyngeal skeleton size, because with severe loss of function of the pathway, particularly the ventral elements of the skeleton can be dramatically reduced. Indeed, the early studies of Edn1 signaling mutants in mouse showed loss of function of Edn1, Ednra, or Ece-1, which respectively encode the ligand, receptor, and a ligand processing enzyme, all result in a severely reduced mandible [17], [18], [19], [20]. These reports discuss the function of the pathway as being important for growth or survival of cells in the ventral arches rather than emphasizing regulation of DV patterning. In chick, inhibition of the Ednra receptor through pharmacological methods results in severe reduction of the lower beak and absence of the arch 2-derived hyoid bone [21]. Moreover, loss of a specific Edn1 downstream target gene in mouse, Hand2 results in hypoplastic first and second arches [5], [22]. Zebrafish edn1 and hand2 mutants also have severe reduction of the arch 1 and 2 ventral skeleton [6], [12]. Furthermore, Walker et al. [23] described a substantial reduction in DV elongation of the ventral region of the embryonic pharyngeal arches in zebrafish edn1 and in furina mutants in which maturation of the Edn1 signaling peptide is disrupted. However, it is unknown whether the phenotype is due to change in growth versus morphogenesis.

In this study we use edn1 and hand2 mutants to focus on pharyngeal arch size regulation and examine edn1;hand2 double mutants to learn the epistatic relationships between these two genes. We extend the previous results showing edn1-dependent DV expansion, and we find that the expansion is due to growth, i.e., arch increase in size, rather than morphogenetic shape change. Previous work in zebrafish had demonstrated that edn1 functions upstream to hand2 in a positive pathway regulating DV patterning [6], hence we were surprised to find that in the early pharyngeal arches, hand2 functions as a negative regulator of edn1-dependent ventral outgrowth. We provide direct evidence that the control of this outgrowth is at least in part by regulation of cell proliferation. Finally, we show that hand2 negatively regulates an anterior morphogenetic cell movement in the ventral first arch. This regulation appears to be independent of edn1 function.

Results

Epistasis Analysis of Larval Cartilage Phenotypes: an edn1–hand2 Genetic Pathway

Previous work has established that with severe loss of function of either edn1 or hand2 in zebrafish, developmental patterning of the embryonic pharyngeal arches is disrupted along the DV axis [6], [10], [12], [24]. Subsequently, the arch-derived early larval skeleton is severely malformed (Figure 1). We focus on the first two pharyngeal arches (arch 1, mandibular; arch 2, hyoid). Heterozygotes, including compound heterozygotes have no discernable mutant phenotypes (not shown). The skeletal phenotypes of homozygous edn1 and hand2 single mutants are essentially as previously described [6], [10], [12], [24], fully penetrant and broadly similar to each other. However, the phenotypes differ in detail. In the second arch in both single mutants, the hyomandibular dorsal region of the hyosymplectic cartilage is almost normal. In contrast, ventrally both single mutants have variable numbers of small cartilage nodules in the place of ventral ceratohyal cartilage, prominent in the wild type (WT), and the ventral midline basihyal cartilage. Intermediate between the dorsal and ventral elements, the WT forms the symplectic and interhyal cartilages and the articulation (DV joint) between the interhyal and ceratohyal. None of these features are present in the edn1 single mutant. In the hand2 single mutant, a recognizable interhyal is absent, but the symplectic and joint are present. Thus it is in this intermediate region where the phenotypes of the two mutants differ.

Download:

Figure 1. edn1 and hand2 are required for ventral jaw cartilage development.

4 dpf zebrafish skeletons were cartilage and bone stained with Alcian Blue and Alizarin Red, dissected and flat-mounted. (A) WT, with cartilages of the first two arches indicated: In the first arch the dorsal palatoquadrate (pq) and ventral Meckel’s cartilage (mk) articulate, Meckel’s cartilage includes a distinctive retroarticular process (ra) adjacent to the joint. In the second arch the more dorsal hyosymplectic cartilage is subdivided into the hyomandibular (hm) and symplectic (sy) regions, and the prominent ventral cartilage is the ceratohyal (ch). The interhyal cartilage (ih) forms a small hinge within the joint region. (B) In the edn1⁻ larva, ventral cartilages and elements of the joint regions are missing or prominently disrupted. Unidentifiable elements are scattered near the ventral midline. (C) The hand2⁻ larva exhibits ventral reductions similar to edn1⁻, but the arch 2 symplectic cartilage and joint (arrow) are present and the arch 1 retroarticular process is expanded rather than missing. (D) The edn1⁻;hand2⁻ larva exhibits defects similar to edn1⁻; in particular, the symplectic cartilage and retroarticular process cannot be identified. Anterior is upward and right is towards the left. Scale bar: 100 µm.

https://doi.org/10.1371/journal.pone.0067522.g001

As we interpret the first arch phenotypes of both single mutants, we also reach the conclusion that the mutants differ in the intermediate region. The dorsal pterygoid process and upper palatoquadrate cartilages are present in both single mutants. Ventrally in both, Meckel’s cartilage is extremely reduced. The intermediate region in WT forms the joint between the palatoquadrate and Meckel’s elements and a prominent retroarticular region of Meckel’s cartilage adjacent to the joint. In the edn1 mutant both features are absent. In the hand2 mutant the joint is absent, but in the territory of the retroarticular process we see a locally expanded wedge- or fan-shaped region of cartilage, previously interpreted as being dorsalized [10]. Not shown in this preparation, the bilateral fan-shaped regions often meet in the midline [10].

The zebrafish edn1;hand2 double mutant has not been previously described. The most striking aspect is its overall phenotypic resemblance to the edn1 single mutant. This finding is consistent with previous understanding that the two genes act positively with respect to ventral cartilage development, and that they function on the same genetic pathway [10], [12]. We do not see a substantially more severe phenotype that might result in the double mutant if the genes were on two different pathways and interacted synergistically. In the intermediate regions of both arches, where the single mutant phenotypes differ, the double mutant phenotype clearly most resembles the edn1 mutant rather than the hand2 mutant. In the second arch, the symplectic and joint are absent. Strikingly, in the intermediate region of the first arch where the single mutants perturb the WT condition in opposite directions (a reduction of cartilage in edn1⁻ versus a local expansion in hand2⁻) we also see an edn1⁻ -like reduction, showing that for this phenotype edn1 is epistatic to hand2. This finding indicates that the relationship between the two genes is complex, seemingly in opposite directions for the positive interaction responsible for overall cartilage reduction and for the negative interaction in expansion in the first arch intermediate region (see Discussion).

A Novel Interaction between edn1 and hand2 in the Embryonic Pharyngeal Arches

To explore the developmental basis of edn1– hand2 interaction, we examined expression of fli1a:EGFP, a marker of neural crest derived ectomesenchyme, during early pharyngula stages (at 24, 28, and 32 hours postfertilization (hpf)). At these stages patterning genes under control of edn1, including hand2, are transcriptionally upregulated and likely functional [12]. Walker et al., using dlx2a expression as a proxy for arch morphology, discovered an edn1 mutant arch phenotype that becomes apparent during this period – a ventral-specific reduction in the DV extent of the pharyngeal arches, which normally are rapidly extending along this axis [23]. At 24 hpf we find no differences in arch morphologies between the WT, the edn1 and hand2 single mutants, and the edn1;hand2 double mutant (Figure 2, first row of panels). However, within the next four hours, prominent DV extension has occurred in the WT (compare Figure 2A1 and A2), and still more prominently in the hand2 mutant (Figure 2C1 and C2). In contrast, there is reduced DV extension in the edn1 single mutant (Figure 2B1 and B2, matching our earlier findings [23]). The 28 hpf DV extension in the edn1;hand2 double mutant phenotype (Figure D2) is similar to that of the edn1 single mutant, and note that the reduction in these mutants is opposite to the expansion in the hand2 single mutant (Figure 2C2). These relations persist at the 32 hpf stage (third column of panels in Figure 2; Figure 3).

Download:

Figure 2. edn1 and hand2 are required for proper growth and morphogenesis of the early pharyngeal arches.

Projections of lateral confocal images of embryos expressing fli1a:EGFP taken at 24, 28, and 32 hpf. This figure provides an overview of changes in the first two arches (a1, a2, separated by the first pharyngeal pouch, p) that are quantified and more fully documented in subsequent figures. Dorsal is to the top in each panel, and anterior is to the left. No differences in arch morphology are observed among the four genotypes at 24 hpf (upper row of panels). Subsequently the arches prominently lengthen along the DV axis; this DV extension is evidently reduced in the edn1 mutant (B2,B3) and edn1;hand2 double mutant (D2,D3) compared to WT and the hand2 mutant. The arches (particularly the first), also shorten along the AP axis but there appears to be no differences in AP shortening among the genotypes. The hand2 mutant also shows marked expansion of mesenchyme ventral to the stomodeum (s) in the anterior first arch (C2,C3). Scale bar: 50 µm.

https://doi.org/10.1371/journal.pone.0067522.g002

Download:

Figure 3. Counterstaining the fli1a:EGFP-expressing pharyngeal arches (a1, a2) with the nucleic acid stain SYTO 59 (red) clarifies the ectomesenchymal phenotypes (double-labeled).

The DV ventral extension differences (arrowheads) are apparent ventral to the red-stained first pharyngeal pouch (p). Compared to the WT (A) this ventral region of mesenchyme is reduced in the edn1 mutant (B) and double mutant (D), and expanded in the hand2 mutant (C). Anterior extension of mesenchyme ventral to the stomodeum (s) is prominent in the hand2 mutant and double mutant (*, C, D).

https://doi.org/10.1371/journal.pone.0067522.g003

At two levels along the AP axis, we can learn whether the differences in DV extension of the arches are predominantly due to changes of the more ventral region of ectomesenchyme. One of the regions, examined previously [23], is the border region between the first and second arches, ventral to the first pharyngeal pouch (arrowheads in Figure 3). The second region is the anterior part of the first arch, where the invaginated oral ectoderm, the stomodeum, is ventrally underlain by the ectomesenchyme (Figure 3C, D; asterisk). In both of these regions epithelium forms a dorsal border to the mesenchyme, providing for quantification of the amounts of DV extension of these ventral mesenchymal regions. Such measurements in sets of 28 hpf genotyped embryos reveals that in both locations the edn1 mutant phenotype has a significant reduction of the ventral mesenchyme compared with WT, the hand2 mutant has an expansion, and the double mutant matches edn1, showing edn1 to be the epistatic gene (Figure 4A, B). We note that these early phenotypes, as well as the epistatic relationship, are just the same as for the later first arch intermediate region skeletal phenotypes described above.

Download:

Figure 4. Quantification of the DV extension phenotypes supports edn1 being epistatic to hand2 in a single regulatory pathway.

DV-length measurements were made for each group, beneath the end of the invaginated stomodeum (A) and beneath the first pharyngeal pouch (B, location indicated by arrowheads in Figure 3). In both locations, and compared to the WT, the edn1 mutant shows reduced DV extension, the hand2 mutant shows increased DV extension and the double mutant most closely resembles the edn1 mutant. Tukey-Kramer analysis supports these three groupings as being significantly different (P<0.05), whereas the differences between edn1⁻ and the double mutant are insignificant.

https://doi.org/10.1371/journal.pone.0067522.g004

The Pharyngeal arch DV Extension Phenotypes are likely due to Changes in arch Size

Two prominent possibilities for the differences in morphology we observed are that the cell arrangements in the pharyngeal arches differ according to genotype, hence giving rise to different arch shapes without a change in size, and/or that arch sizes are different, e.g., through changes in cell growth or death. We used several approaches to examine these possibilities.

Cell rearrangement could underlie convergence and extension of the arches during the early pharyngula period, evident from the time course shown in Figure 2. At 24 hpf the arches are not only very short along the dorsal-ventral axis, but they are also prominently elongated along the AP axis. By 28 hpf they have converged, i.e., shortened, along the AP axis and extended, or lengthened, along the DV axis. Do the arch shapes differ significantly according to genotype at this stage? We used the sensitive methods of landmark-based geometric morphometrics [25], [26], including a Principal Component Analysis (PCA) to compare the shapes of the arches. Plotting PC1 by PC2 yields a ‘shape space’ accounting for about 57% of the total shape variation (Figure 5). As shown by the shape configuration diagrams accompanying the plot, PC1 prominently captures the overall lengths along the DV axis of both arches, DV lengthening at positive PC1 values, and shorting at negative PC1 values. PC2, in contrast, primarily accounts for a more local change in the amount of tissue ventral to the stomodeum in the first arch (the region examined in Figure 4B). Notably, at this 28 hpf time point neither PC1 nor PC2 reveal substantial variation associated with arch lengths along the AP axis. If the basis of the shape change revealed by the PCA were due to AP convergence coupled with DV extension, we would expect an AP change to be detected by the PCA. Hence the findings suggest that the differences between genotypes with low PC1 values (edn1 mutants and the double mutants), and high PC1 values (WT and hand2 mutants) are not due to convergence and extension. The data do not show that arch convergence and extension is absent at this stage, only that the four genotypic groups do not differ from one another in this respect. Indeed, following the time course of changes by PCA suggests that the early arches are indeed undergoing convergence and extension, and that the genotype-specific changes occur progressively with time (Figure S1).

Download:

Figure 5. Quantification of arch morphology by PCA reveals that edn1 and hand2 regulate two prominent features of arch shape, DV extension (PC1) and ventral arch 1 anterior extension (PC2).

Together these two deformations account for 58% of the total shape variation within the dataset, which uses landmarks (numbered in the accompanying wireframe diagrams) to outline the fli1a:EGFP-expressing tissue of the first two pharyngeal arches at 28 hpf. Shape change along the AP axis is minimal. We interpret the nature of the shape changes from the wireframes. For each, the light blue wireframe shows the consensus configuration and the dark blue wireframe shows the deformation associated with change (+ or -) along a PC axis. In the plot itself the individual measurements are grouped by genotype with a different color and 95% ellipses for each (sampling 23 or more individuals in each group). The data show overlap among the groups, yet Procrustes distance measurements reveal all the groups are significantly different from one another (P<0.0001 by permutation; data not shown). WT and the hand2 single mutant score high on PC1, whereas the edn1 single mutant and the double mutant score low on PC1. WT and the edn1 mutant score high on PC2, whereas the hand2 mutant and the double mutant score low. Hence the double mutant phenotype is additive in this analysis, combining the shape features of both single mutants.

https://doi.org/10.1371/journal.pone.0067522.g005

Size variation is factored out of these geometric morphometric analyses (Figure 5), which examine only shape variation. Nevertheless, we interpret the PCA to mean that size change accounts for the changes in DV extension. We hypothesize that the genotype-specific differences revealed by PC1 specifically are simply accounted for by how much arch mesenchyme is present at this stage in the arches globally and/or in the ventral regions specifically. To test the hypothesis directly we measured the volumes of the arches, and predicted that arch volume should be greater in the hand2 mutant relative to WT, less in the edn1 mutant, and less than WT in the double mutant as well. No such changes in volume are predicted by the alternative, morphogenetic movement hypothesis. Quantitative estimates of the combined arch 1 and 2 volumes of regions of fli1a:EGFP-expressing mesenchyme, match these predictions (Figure 6A).

Download:

Figure 6. edn1 positively and hand2 negatively regulate the volume of pharyngeal arch fli1a:EGFP expressing mesenchyme (A) and ventral domain proliferation of neural crest derived cells (B–E).

Data are for 28 hpf, a minimum of 23 individuals of each genotype were sampled. (B) shows an example 2-color image of phospho-histone H3 labeling for mitosing cells (red) and fli1a:EGFP expression (green). (C–E) show mean counts of double-labeled cells ±SEM. Tukey-Kramer comparison of the mean volumes (in A) reveals that the edn1 mutant volume is significantly lower than WT, and that the hand2 mutant volume is significantly higher (P<0.05). Statistically the double mutant phenotype is neither different from the edn1 mutant nor WT, suggesting some degree of phenotypic rescue of arch volume when hand2 does not function. Tukey-Kramer analysis of the levels of proliferation in both the total mesenchyme (C) and ventral sector of mesenchyme (E) reveals three statistically distinctive classes, WT, the single hand2 mutant, and the single edn1 plus edn1;hand2 mutant class (P<0.05). Genotypic differences for the dorsal mesenchyme (D) are insignificant.

https://doi.org/10.1371/journal.pone.0067522.g006

edn1 and hand2 Interact to Control Cell Proliferation in the Ventral Pharyngeal Arches

The changes in the volumes of the neural crest-derived portions of the 28 hpf arches described above might arise through a variety of mechanisms, including differences in recruitment, cell death, cell size, or cell proliferation. We could not meaningfully test cell size because of the very tight packing of cells in the fli1a:EGFP expressing mesenchyme, however there is no indication of a prominent cell-size difference among these genotypes. TUNEL labeling showed that there is essentially negligible programmed cell death in the WT, and this level is not increased in the edn1 mutant (Table S1), matching previous findings with ednra1 and ednra2 knockdown [27]. Additionally, we generated edn1;p53 double mutants, and examined their early larval skeletal phenotypes (Figure S2). We found no phenotypic rescue. Hence, this analysis argues against p53-dependent cell death as an explanation for the reduced size of the arches.

We used phospho-histone H3 labeling to examine proliferation, including fli1a:EGFP as a second label to mark neural crest derived mesenchyme (Figure 6B). Double-labeled cells are present in both dorsal and ventral sectors of the arches (Figure 6B). Strikingly, the relative levels of proliferating ectomesenchymal cells within the total combined arch1 and 2 for each genotype are similar to those for arch volume (Figure 6C, compare with A). The differences between the single mutants are even more striking when proliferation in just the ventral part of the arches is compared, and the double mutant is statistically indistinguishable from the edn1 single mutant (Figure 6E). Genotype-specific differences are less prominent in the dorsal sector (Figure 6D). These finding suggest that changes in the volume of ectomesenchyme in the pharyngeal arches that are associated with genotype are at least in part due to differences in cell proliferation, primarily occurring in the ventral regions. For all of these phenotypes, edn1 and hand2 exert their controls in opposite directions (positive versus negative) and the epistasis between the two genes is the same; edn1 is epistatic to hand2.

hand2 Regulates Anterior Extension in the Ventral First arch in an edn1-independent Manner

Besides DV expansion of the ventral arches, as noted above we observed a prominent anterior extension of the ventral first arch shared by the hand2 single mutant and the edn1;hand2 double mutant (Figure 2; and the anterior extension is captured by PC2 in Figure 5 and Figure S1). This change is due to an expansion in the region ventral to the stomodeum, as might be due to a flow of cells into this ventral territory. We used time-lapse recordings to examine this hypothesis. We observed that in the WT and in all three mutant conditions there is a distinctive anterior flow of cells within the ventral first arch that serves to anteriorly extend the region singled out by PC2 (Figure 7, movie S1). This anterior extension movement is much more prominent in the hand2 mutant and in the double mutant than in both WT and the edn1mutant. Following the courses of individual cells in the ventral arch (Figure 7, movie S1; arrows) strongly supports this inference. Our recordings suggest that WT and the edn1 mutant form a single phenotypic class in which the anterior extension movement is relatively slow, whereas the hand2 and double mutant share another class with much more rapid movement. We interpret these findings to mean that hand2 functions as a negative regulator of this anterior extension cellular movement in the ventral first arch, and that edn1 plays no role in this regulation.

Download:

Figure 7. hand2 negatively regulates anterior flow of ventral arch 1 cells.

fli1a:EGFP animals were imaged by time lapse microscopy from 24–32 hpf. Panels are excerpts from the movie S1 in which maximum confocal projections are presented. Red balls represent the location of an individual cell that was manually tracked in each frame. The positions of tracked cells are overlaid in the outlines. Cells travel from near the midpoint of arch1 to a location posterior to the stomodeum and the eye in wild types and edn1 mutants (A, B). Cells originating at a similar location in hand2 and hand2;edn1 double mutants travel much further, to a position well under the stomodeum and the eye (C, D). Scale bar: 50 µm.

https://doi.org/10.1371/journal.pone.0067522.g007

Discussion

Previous studies on the role of the Edn1 signaling pathway in development have mostly focused on the regulation of developmental patterning in the anterior pharyngeal arches: how are separate skeletal elements and their articulating joints specified in a position-dependent manner? Here we focused primarily on growth and morphogenesis in the embryonic pharyngeal arches. In doing so, we discovered a novel genetic interaction between edn1 and hand2. This interaction shows itself in the control of very early DV outgrowth in the ventral arches during the pharyngula period of embryonic development. The control is mediated, at least in part, through edn1-dependent cell proliferation. However, we cannot rule out alternative mechanisms such as recruitment of additional cells to express fli1a:EGFP. Also novel is that we discovered edn1 to be epistatic to hand2 in a negative genetic interaction controlling this outgrowth and proliferation. In contrast, previous studies in zebrafish and mouse support both edn1 and hand2 as being positive, not negative, effectors of ventral arch outgrowth and differentiation. Finally, we show that hand2 acts as a negative regulator of a previously undescribed morphogenetic movement that sweeps cells forward in an anterior direction within the ventral first pharyngeal arch. edn1 appears to play no role in this ‘anterior extension’ cell movement, at least at the early stages of arch morphogenesis we examined.

hand2 as a Negative Regulator of edn1-dependent Cell Proliferation

We find that one edn1 function is to promote early expansion of the ventral regions of the pharyngeal arches by upregulating local proliferation, and that this action is blocked by hand2. Consistent with previous zebrafish results with knockdowns of the ednra receptors [27], we find TUNEL labeling of cells in the zebrafish pharyngeal arches to be rare, and no change in either the edn1 or hand2 single mutant, suggesting that the cell death pathway is not involved in size regulation. These data contrast with some from other vertebrates suggesting Edn1 and Hand2 function positively together to regulate growth in arch size through inhibiting cell death [5], [7], [28], [29]. However, this mechanism remains controversial as work with Hand2 conditional knockouts [13] suggests the cell death observed in Hand2 conventional knockouts [5] may be due to loss of embryo viability, as opposed to a more direct function of Hand2 in preventing cell death. Another possibility accounting for the difference between our data and those from other models is timing, for we focused on an early eight hour interval in the embryo when the mutant phenotypes are only first showing up. From the larval skeletal phenotypes it is likely that size regulation changes dynamically during arch development (discussed further below). We also note that in in vitro studies in human cancer cell lines EDN1 promotes cell proliferation as well as inhibiting cell death [30], [31], [32].

edn1 being epistatic to hand2 in the control of early proliferation would place hand2 genetically upstream of edn1, were their interaction within a linear genetic pathway [33]. In contrast, RNA in situ evidence is clear that edn1 is molecularly upstream of hand2 [6]. This apparent paradox can be easily accommodated by understanding that there is cross-talk among edn1-target genes [10], [12]. Hence genetic interaction is likely within a network, such as we propose in Figure 8A, rather than within a linear pathway. In fact, identical negative regulatory circuitry to that in Figure 8A has already been proposed: Dlx genes function in the intermediate domain under positive control of edn1 as demonstrated by their downregulation in edn1 mutants [6], [11], [12], [23], and the Dlx genes are negatively regulated by hand2, as demonstrated by their upregulation in hand2 mutants [10], [13] The edn1-hand2-Dlx interaction thus provides precedent for our model in Figiure 8A, and indeed it is possible that Dlx genes themselves mediate the regulation of early proliferation that our model requires. Talbot et al. described the expansion of the ventral-anterior region of the first pharyngeal arch in the zebrafish hand2 mutant being accompanied by an expansion of the intermediate domain Dlx genes [10]. Testing whether hand2– Dlx gene interaction is involved in ventral proliferation is likely possible with currently available methods, but would be difficult because of redundancy of function of Dlx genes (including dlx3b, dlx4a and dlx5a [10]), and lack of suitable loss of function mutants. Another class of homeobox genes, Msx genes, might also function as downstream effectors of edn1-dependent control cell proliferation; expression of at least two such genes are under positive control of edn1 and negative control by hand2 [12].

Download:

Figure 8. Regulatory genetic network for control of growth and morphogenesis in the pharyngeal arches by edn1 and hand2.

(A) The model assumes that regulation of early proliferation in the ventral arches, in which edn1 is epistatic to hand2, can account for the DV extension phenotype explored in this study. The positive pathway regulating patterning and late outgrowth accounts for the general reduction of elements in the ventral skeleton, as well skeletal disruption because of downregulation of downsteam patterning genes studied elsewhere [10], [12], [23], [24]. This model predicts a temporally dynamic switching in hand2 function, from negative to positive, which can be explored in future studies. (B) We propose hand2 negatively regulates the anterior extension movement in the ventral first arch independent of edn1 function.

https://doi.org/10.1371/journal.pone.0067522.g008

Our finding of negative interaction between edn1 and hand2 would at first glance be at odds with the previous understanding of positive interaction in zebrafish. The earlier model derives in part from the finding that the ventral elements of the early larval skeleton are generally reduced, hypoplastic, with loss of function of either of the two genes. In examining the early larva we also observe generalized ventral skeletal hypoplasia in all three mutant conditions we addressed, confirming the earlier work. Our model incorporates the positive interaction simply by adding a branch to the network (the downward branch in Figure 8A). The key difference between the two output branches of the network is likely one of timing, i.e., hand2 regulation switches from negative to positive at stages later than the 24–32 hpf stages we examined here. In support, aspects of hand2 function have already been shown to be dynamic during embryonic pharyngeal arch development [15], [23], [24].

How does Control of Early Pharyngeal arch Phenotype Relate to the Later Cartilage Phenotype?

We observed that even though Meckel’s cartilage is severely reduced in hand2 mutant larvae, matching previous studies [10], [12], there is a local size increase in this cartilage’s retroarticular process [10], [24]. The retroarticular region is that part of the cartilage nearest to the joint, i.e., the most dorsal or proximal region of this element. The retroarticular is not distinguished in the overall massively reduced Meckel’s cartilage of the edn1 mutant, and the edn1;hand2 double mutant matches the edn1 mutant in this respect.

We propose that developmental regulation of the size of this most proximal region of the ventral cartilage occurs at the very earliest stages of pharyngeal arch development after neural crest migration. This is the time period when we have shown that negative control by hand2 is exerted. This hypothesis predicts that the most proximal region of Meckel’s cartilage, a region within the intermediate domain of patterning [10] might be the developmentally oldest region of the cartilage. We do not know if the ventral cartilages grow out in some temporally-specific proximal-to-distal sequence, as could be examined in future studies.

hand2 Negatively Regulates edn1-independent Morphogenetic Movement

In addition to the DV outgrowth regulation just discussed, we observed a negative regulation by hand2 of an anterior extension in the ventral first arch, most likely independent of edn1 function (Figure 8B). Whereas our evidence strongly points to DV outgrowth being due to cell proliferation, morphogenetic movement is just as clearly the primary cause of anterior extension; our time lapse recordings show movement of ventral mesenchymal cells across the arch, flowing into the region of the stomodeum, and underneath the stomodeum. The recordings, along with our PCA, suggest this movement is specific to the ventral first arch; finding that cells move within the arch itself suggests active cellular migration. While it is possible that subtle changes in this morphogenesis are present in edn1 mutants, we are unable to detect any edn1 dependent differences in our time lapse analyses. Interestingly, some Hand2 expression domains are apparently independent of Edn1 signaling in both zebrafish and mice [6], [8], and we propose that the small amount of hand2 expressing cells that remain in edn1 mutants are competent to prevent the morphogenetic movement. In fact, ectopic BMP can induce hand2 expression in the absence of edn1 [15], a precedent for hand2 functioning independent of edn1 in ventral arch1 development.

The time-lapse recordings also show a prominent anterior movement of the second arch, but not its narrowing, and seemingly not cells moving within the arch as for the first. Hence we interpret the second arch movement as being passively imposed by the first, to which it is connected through ventral mesenchyme. That cell migration is specific to the first arch makes sense functionally because of the way the invaginated oral ectoderm forms a barrier preventing ventrally migrating neural crest from populating the ventral anterior region of the arch directly: The anterior movement is required for the development of the lower jaw. No such epithelial barrier exists in the second or more posterior arches. We note that micrognathia is a relatively common human craniofacial disorder, a part of many syndromes (e.g, DiGeorge [OMIM188400], Treacher-Collins [OMIM154500],) and not well understood. It could well be that some specific instances of the human disorder could involve partial failure of anterior extension.

Our work not only identifies Edn1 as a growth factor in pharyngeal arch development, but particularly highlights the complexity of regulation involving hand2, both in terms of signaling pathways that converge on hand2 and in its role as a focal point in the regulation of downstream effector genes mediating a variety of functions – patterning [10], [15], as well as growth and morphogenesis (Figure 8). In particular, our study demonstrates the value of the zebrafish model in allowing precise investigation of the cellular events occurring during early pharyngeal arch development, and how specific cellular behaviors depend on the developmental regulatory gene environment.

Materials and Methods

Fish Stocks and Maintenance

Fish were raised under standard conditions [34] and staged as described [35]. The following lines have been previously described: edn1^tf216b [6], Df(Chr01:hand2)s6 [36], Tg(fli1a:EGFP) [37], p53^zdf1 [38]. Heterozygous lines were maintained on an inbred AB genetic background. edn1⁻ was identified using forward primer: 5′ GGTGCTCCAGCATCTTTGGGTC3′ and reverse primer: 5′TGTCTGTTCTGACTTACTCTGGTG3′ resulting in a 153 bp product. Digestion with MseI cleaved the PCR product from the mutant allele into 84 and 69 bp fragments. hand2⁻ was identified by PCR using forward primer: 5′ GCGGACAGTGAAACGTAGACC 3′ and reverse primer: 5′ GCCTTTCTTCTTTGGCGTCTGTC 3′ resulting in a 257 bp product from the WT allele. p53⁻ was genotyped as described [38] All of our work with zebrafish has been approved by the University of Oregon Institutional Animal Care and Use Committee (IACUC). Assurance number for animal research: A-3009-01.

Skeletal Staining and Morphometric Analysis

Larvae were fixed at 4 or 6 days postfertilization (dpf) and stained with Alcian Blue for cartilage and Alizarin Red for bone as described [39], [40].

Microscopy

Skeletal preparations were imaged on a Zeiss Axiophot 2. Static confocal images were captured on a Zeiss LSM 5 Pascal as previously described [41]. Briefly, embryos were manually dechorionated, anesthetized with tricaine and fixed in 4% paraformaldehyde in PBS overnight at 4°C. A piece of the tail was removed and used for genotyping each sample. Embryos were washed with PBS and transferred to 6% methylcellulose on a microscope slide. Z-stacks totaling approximately 90 µm were imaged at 1.5–2.5 µm intervals. For time-lapse movies, animals were mounted and imaged as described [24], [42] on a Leica SD6000 spinning disk confocal. Movies were assembled using Metamorph (Molecular Devices) and ImageJ.

Geometric Morphometric and Volume Analyses

Confocal images taken at 24, 28, and 32 hpf were corrected for orientation using 3D rendering in Volocity (PerkinElmer). For geometic morphometric analysis, twenty landmarks outlining the fli1a:EGFP expressing ectomesenchyme of the first two pharyngeal arches (PAs) were digitized at the positions shown in Figure 5 using tps Dig, version 2.04 software [43]. Further analyses were done in MorphoJ [25], [26]. The data were Procrustes aligned to remove size, rotation, and translation effects, and the shapes analyzed by PCA and Discriminant Function Analysis. Combined volumes of these two arches were measured using Volocity. Regions of interest were established around the anterior PAs and volume measurements were of regions expressing fli1a:EGFP. To provide a counterstain showing total cells within the arches (as in Figure 3), the embryos were incubated with the nucleic acid stain SYTO 59 (Invitrogen) at a 1∶1000 dilution in PBSTx (1% Triton X-100 in 1x PBS) for 1 hour at room temperature. The embryos were washed for 15 minutes with PBSTx at room temperature.

Cell Proliferation Assay

Proliferating cells were detected using anti-phospho-histone H3 antibody. Embryos were manually dechorionated, anesthetized with tricaine, and fixed in 4% paraformaldehyde in PBS overnight at 4°C. Prior to staining, embryos were washed with PBSTx and blocked in 10% normal goat serum (NGS) in PBDTx (0.1% Triton X-100, 1% DMSO, 1% BSA in 1x PBS) for at least 2 hours. Embryos were incubated with rabbit anti-phospho-histone H3 (Millipore) at 1∶1000 dilution in blocking solution overnight at 4°C, washed with PBSTx, then incubated with Alexafluor 546 goat anti-rabbit IgG (Invitrogen) at 1∶500 dilution in PBSTx overnight at 4°C. Samples were visualized by confocal microscopy. Phospho-histone H3 positive cells were detected with Volocity. Regions of interest were set around the PAs and only cells positive for both phospho-histone H3 and fli1a:EGFP were counted.

Cell Death Assay

TUNEL assay was performed to detect cell death. Embryos were dehydrated in 100% MeOH for 1 hour at -20°C then rehydrated by sequential incubation with 75%, 50%, and 25% MeOH in PBSTx at −20°C and with PBSTx at RT for 10 minutes each. Embryos were permeabilized by incubation in Proteinase-K (1 µg/mL) then fixed in 4% PFA for 20 minutes. Embryos were further permeabilized in Permeabilization Solution (0.1% Triton X-100, 0.1% sodium citrate) for 30 minutes then washed with PBSTx. DNA fragmentation was detected by incubation with terminal deoxynucleotidyl transferase and TMR dUTP for 1 hour at 37°C (Roche). Embryos were washed in PBSTx then imaged.

Supporting Information

Figure S1.

The distinctive pharyngeal arch shapes of WT, edn1 and hand2 mutants arise progressively from 24 hpf to 32 hpf. PCA as in Figure 5 of the main text, but here aligned separately for this developmental age series. Nevertheless this PCA and that shown in Figure 5 capture largely the same shape changes, as revealed by comparing the wireframes in each figure. A: PC2 by PC1 scatter plot with all of the individual samples plotted (a minimum of 20 in each of the nine groups). Gray-black filled circles represent WT, pink-red rectangles represent edn1 mutants, and light to dark blue triangles represent hand2 mutants. B. The same plot but showing the means for each genotype-age group. At the 24 hpf time point the three genotypes completely overlap. DV extension, captured by PC1, then increases markedly with developmental age for all genotypes, with edn1⁻ lagging behind WT and hand2⁻. The hand2 mutant shows progressive expansion in the ventral-anterior arch 1 region captured by negative PC2, whereas WT and edn1⁻ show slight change in the opposite direction.

https://doi.org/10.1371/journal.pone.0067522.s001

(TIF)

Figure S2.

Loss of function of the programmed cell death gene p53 does not rescue the skeletal phenotype of the edn1 mutant. Flat-mount of cartilage and bone stained with Alcian Blue and Alizarin Red. The skeletal phenotypes of the edn1 single mutant and the edn1;p53 double mutant appear identical, whereas phenotypic rescue would be expected if programmed cell death of pharyngeal arch precursor cells accounted for the edn1⁻ hypoplastic skeleton. Hence the experiment argues against cell death as an explanation for the reduced size of the arches.

https://doi.org/10.1371/journal.pone.0067522.s002

(TIF)

Table S1.

TUNEL labeling to detect cell death in the pharyngeal arches.

https://doi.org/10.1371/journal.pone.0067522.s003

(DOCX)

Movie S1.

hand2 negatively regulates anterior flow of ventral arch 1 cells. fli1a:EGFP animals were imaged by time lapse microscopy from 24–32 hpf. Movies are confocal projections in which individual cells were manually tracked at each frame (arrow). Cells travel from near the midpoint of arch1 to a location posterior to the stomodeum and the eye in wild types and edn1 mutants (A, B). Cells originating at a similar location in hand2 and hand2;edn1 double mutants travel much further, to a position well under the stomodeum and the eye (C, D). Scale bar: 50 µm

https://doi.org/10.1371/journal.pone.0067522.s004

(MOV)

Acknowledgments

We would like to thank John Dowd and the University of Oregon fish facility for exceptional animal care.

Author Contributions

Conceived and designed the experiments: JTN CBK MMS. Performed the experiments: JTN MMS. Analyzed the data: JTN CBK MMS. Wrote the paper: JTN MMS CBK. Contributed equally to this work: JTN MMS.

References

1. Schilling TF, Piotrowski T, Grandel H, Brand M, Heisenberg CP, et al. (1996) Jaw and branchial arch mutants in zebrafish I: branchial arches. Development 123: 329–344.
- View Article
- Google Scholar
2. Piotrowski T, Schilling TF, Brand M, Jiang YJ, Heisenberg CP, et al. (1996) Jaw and branchial arch mutants in zebrafish II: anterior arches and cartilage differentiation. Development 123: 345–356.
- View Article
- Google Scholar
3. Clouthier DE, Schilling TF (2004) Understanding endothelin-1 function during craniofacial development in the mouse and zebrafish. Birth Defects Res C Embryo Today 72: 190–199.
- View Article
- Google Scholar
4. Kimmel CB, Walker MB, Miller CT (2007) Morphing the hyomandibular skeleton in development and evolution. J Exp Zool B Mol Dev Evol 308: 609–624.
- View Article
- Google Scholar
5. Thomas T, Kurihara H, Yamagishi H, Kurihara Y, Yazaki Y, et al. (1998) A signaling cascade involving endothelin-1, dHAND and Msx1 regulates development of neural-crest-derived branchial arch mesenchyme. Development 125: 3005–3014.
- View Article
- Google Scholar
6. Miller CT, Schilling TF, Lee K, Parker J, Kimmel CB (2000) sucker encodes a zebrafish Endothelin-1 required for ventral pharyngeal arch development. Development 127: 3815–3828.
- View Article
- Google Scholar
7. Clouthier DE, Williams SC, Yanagisawa H, Wieduwilt M, Richardson JA, et al. (2000) Signaling pathways crucial for craniofacial development revealed by endothelin-A receptor-deficient mice. Dev Biol 217: 10–24.
- View Article
- Google Scholar
8. Ruest LB, Xiang X, Lim KC, Levi G, Clouthier DE (2004) Endothelin-A receptor-dependent and -independent signaling pathways in establishing mandibular identity. Development 131: 4413–4423.
- View Article
- Google Scholar
9. Ruest LB, Clouthier DE (2009) Elucidating timing and function of endothelin-A receptor signaling during craniofacial development using neural crest cell-specific gene deletion and receptor antagonism. Developmental Biology 328: 94–108.
- View Article
- Google Scholar
10. Talbot JC, Johnson SL, Kimmel CB (2010) hand2 and Dlx genes specify dorsal, intermediate and ventral domains within zebrafish pharyngeal arches. Development 137: 2506–2516.
- View Article
- Google Scholar
11. Tavares ALP, Garcia EL, Kuhn K, Woods CM, Williams T, et al. (2012) Ectodermal-derived Endothelin1 is required for patterning the distal and intermediate domains of the mouse mandibular arch. Developmental Biology 371: 47–56.
- View Article
- Google Scholar
12. Miller CT, Yelon D, Stainier DY, Kimmel CB (2003) Two endothelin 1 effectors, hand2 and bapx1, pattern ventral pharyngeal cartilage and the jaw joint. Development 130: 1353–1365.
- View Article
- Google Scholar
13. Barron F, Woods C, Kuhn K, Bishop J, Howard MJ, et al. (2011) Downregulation of Dlx5 and Dlx6 expression by Hand2 is essential for initiation of tongue morphogenesis. Development 138: 2249–2259.
- View Article
- Google Scholar
14. Zuniga E, Stellabotte F, Crump JG (2010) Jagged-Notch signaling ensures dorsal skeletal identity in the vertebrate face. Development 137: 1843–1852.
- View Article
- Google Scholar
15. Zuniga E, Rippen M, Alexander C, Schilling TF, Crump JG (2011) Gremlin 2 regulates distinct roles of BMP and Endothelin 1 signaling in dorsoventral patterning of the facial skeleton. Development 138: 5147–5156.
- View Article
- Google Scholar
16. Alexander C, Zuniga E, Blitz IL, Wada N, Le Pabic P, et al. (2011) Combinatorial roles for BMPs and Endothelin 1 in patterning the dorsal-ventral axis of the craniofacial skeleton. Development 138: 5135–5146.
- View Article
- Google Scholar
17. Kurihara Y, Kurihara H, Suzuki H, Kodama T, Maemura K, et al. (1994) Elevated blood pressure and craniofacial abnormalities in mice deficient in endothelin-1. Nature 368: 703–710.
- View Article
- Google Scholar
18. Clouthier DE, Hosoda K, Richardson JA, Williams SC, Yanagisawa H, et al. (1998) Cranial and cardiac neural crest defects in endothelin-A receptor-deficient mice. Development 125: 813–824.
- View Article
- Google Scholar
19. Yanagisawa H, Yanagisawa M, Kapur RP, Richardson JA, Williams SC, et al. (1998) Dual genetic pathways of endothelin-mediated intercellular signaling revealed by targeted disruption of endothelin converting enzyme-1 gene. Development 125: 825–836.
- View Article
- Google Scholar
20. Abe M, Ruest LB, Clouthier DE (2007) Fate of cranial neural crest cells during craniofacial development in endothelin-A receptor-deficient mice. Int J Dev Biol 51: 97–105.
- View Article
- Google Scholar
21. Kempf H, Linares C, Corvol P, Gasc JM (1998) Pharmacological inactivation of the endothelin type A receptor in the early chick embryo: a model of mispatterning of the branchial arch derivatives. Development 125: 4931–4941.
- View Article
- Google Scholar
22. Srivastava D (1997) Regulation of cardiac mesodermal and neural crest development by the bHLH transcription factor, dHAND (vol 16, pg 154, 1997). Nature Genetics 16: 410–410.
- View Article
- Google Scholar
23. Walker MB, Miller CT, Coffin Talbot J, Stock DW, Kimmel CB (2006) Zebrafish furin mutants reveal intricacies in regulating Endothelin1 signaling in craniofacial patterning. Dev Biol 295: 194–205.
- View Article
- Google Scholar
24. Nichols JT, Pan L, Moens CB, Kimmel CB (2013) barx1 represses joints and promotes cartilage in the craniofacial skeleton. Development In Press.
25. Klingenberg CP (2009) Morphometric integration and modularity in configurations of landmarks: tools for evaluating a priori hypotheses. Evolution & Development 11: 405–421.
- View Article
- Google Scholar
26. Klingenberg CP (2011) MorphoJ: an integrated software package for geometric morphometrics. Molecular Ecology Resources 11: 353–357.
- View Article
- Google Scholar
27. Nair S, Li W, Cornell R, Schilling TF (2007) Requirements for Endothelin type-A receptors and Endothelin-1 signaling in the facial ectoderm for the patterning of skeletogenic neural crest cells in zebrafish. Development 134: 335–345.
- View Article
- Google Scholar
28. Aiyer AR, Honarpour N, Herz J, Srivastava D (2005) Loss of Apaf-1 leads to partial rescue of the HAND2-null phenotype. Developmental Biology 278: 155–162.
- View Article
- Google Scholar
29. Bonano M, Tribulo C, De Calisto J, Marchant L, Sanchez SS, et al. (2008) A new role for the Endothelin-1/Endothelin-A receptor signaling during early neural crest specification. Developmental Biology 323: 114–129.
- View Article
- Google Scholar
30. Bagnato A, Tecce R, DiCastro V, Catt KJ (1997) Activation of mitogenic signaling by endothelin 1 in ovarian carcinoma cells. Cancer Research 57: 1306–1311.
- View Article
- Google Scholar
31. Del Bufalo D, Di Castro V, Birocco A, Salani D, Rosano L, et al. (2002) Endothelin-1 acts as a survival factor in ovarian carcinoma cells. Clinical Science 103: 302S–305S.
- View Article
- Google Scholar
32. Del Bufalo D, Di Castro V, Biroccio A, Varmi M, Salani D, et al. (2002) Endothelin-1 protects ovarian carcinoma cells against paclitaxel-induced apoptosis: Requirement for Akt activation. Molecular Pharmacology 61: 524–532.
- View Article
- Google Scholar
33. Avery L, Wasserman S (1992) Ordering gene function: the interpretation of epistasis in regulatory hierarchies. Trends Genet 8: 312–316.
- View Article
- Google Scholar
34. Westerfield M (1993) The zebrafish book: A guide for the laboratory use of zebrafish (Brachydanio rerio).
35. Kimmel CB, Ballard WW, Kimmel SR, Ullmann B, Schilling TF (1995) Stages of embryonic development of the zebrafish. Dev Dyn 203: 253–310.
- View Article
- Google Scholar
36. Yelon D, Ticho B, Halpern ME, Ruvinsky I, Ho RK, et al. (2000) The bHLH transcription factor hand2 plays parallel roles in zebrafish heart and pectoral fin development. Development 127: 2573–2582.
- View Article
- Google Scholar
37. Lawson ND, Weinstein BM (2002) In vivo imaging of embryonic vascular development using transgenic zebrafish. Dev Biol 248: 307–318.
- View Article
- Google Scholar
38. Berghmans S, Murphey RD, Wienholds E, Neuberg D, Kutok JL, et al. (2005) tp53 mutant zebrafish develop malignant peripheral nerve sheath tumors. Proceedings of the National Academy of Sciences of the United States of America 102: 407–412.
- View Article
- Google Scholar
39. Walker MB, Kimmel CB (2007) A two-color acid-free cartilage and bone stain for zebrafish larvae. Biotech Histochem 82: 23–28.
- View Article
- Google Scholar
40. Eames BF, Yan YL, Swartz ME, Levic DS, Knapik EW, et al. (2011) Mutations in fam20b and xylt1 Reveal That Cartilage Matrix Controls Timing of Endochondral Ossification by Inhibiting Chondrocyte Maturation. Plos Genetics 7.
41. Crump JG, Swartz ME, Kimmel CB (2004) An integrin-dependent role of pouch endoderm in hyoid cartilage development. PLoS biology 2: E244.
- View Article
- Google Scholar
42. Huycke TR, Eames BF, Kimmel CB (2012) Hedgehog-dependent proliferation drives modular growth during morphogenesis of a dermal bone. Development 139: 2371–2380.
- View Article
- Google Scholar
43. Rohlf FJ (2005) tps Dig version 2.04. Stony Brook: Department of Ecology and Evolution, State University of New York.

[ref1] 1. Schilling TF, Piotrowski T, Grandel H, Brand M, Heisenberg CP, et al. (1996) Jaw and branchial arch mutants in zebrafish I: branchial arches. Development 123: 329–344.
View Article
Google Scholar

[2] View Article

[3] Google Scholar

[ref2] 2. Piotrowski T, Schilling TF, Brand M, Jiang YJ, Heisenberg CP, et al. (1996) Jaw and branchial arch mutants in zebrafish II: anterior arches and cartilage differentiation. Development 123: 345–356.
View Article
Google Scholar

[5] View Article

[6] Google Scholar

[ref3] 3. Clouthier DE, Schilling TF (2004) Understanding endothelin-1 function during craniofacial development in the mouse and zebrafish. Birth Defects Res C Embryo Today 72: 190–199.
View Article
Google Scholar

[8] View Article

[9] Google Scholar

[ref4] 4. Kimmel CB, Walker MB, Miller CT (2007) Morphing the hyomandibular skeleton in development and evolution. J Exp Zool B Mol Dev Evol 308: 609–624.
View Article
Google Scholar

[11] View Article

[12] Google Scholar

[ref5] 5. Thomas T, Kurihara H, Yamagishi H, Kurihara Y, Yazaki Y, et al. (1998) A signaling cascade involving endothelin-1, dHAND and Msx1 regulates development of neural-crest-derived branchial arch mesenchyme. Development 125: 3005–3014.
View Article
Google Scholar

[14] View Article

[15] Google Scholar

[ref6] 6. Miller CT, Schilling TF, Lee K, Parker J, Kimmel CB (2000) sucker encodes a zebrafish Endothelin-1 required for ventral pharyngeal arch development. Development 127: 3815–3828.
View Article
Google Scholar

[17] View Article

[18] Google Scholar

[ref7] 7. Clouthier DE, Williams SC, Yanagisawa H, Wieduwilt M, Richardson JA, et al. (2000) Signaling pathways crucial for craniofacial development revealed by endothelin-A receptor-deficient mice. Dev Biol 217: 10–24.
View Article
Google Scholar

[20] View Article

[21] Google Scholar

[ref8] 8. Ruest LB, Xiang X, Lim KC, Levi G, Clouthier DE (2004) Endothelin-A receptor-dependent and -independent signaling pathways in establishing mandibular identity. Development 131: 4413–4423.
View Article
Google Scholar

[23] View Article

[24] Google Scholar

[ref9] 9. Ruest LB, Clouthier DE (2009) Elucidating timing and function of endothelin-A receptor signaling during craniofacial development using neural crest cell-specific gene deletion and receptor antagonism. Developmental Biology 328: 94–108.
View Article
Google Scholar

[26] View Article

[27] Google Scholar

[ref10] 10. Talbot JC, Johnson SL, Kimmel CB (2010) hand2 and Dlx genes specify dorsal, intermediate and ventral domains within zebrafish pharyngeal arches. Development 137: 2506–2516.
View Article
Google Scholar

[29] View Article

[30] Google Scholar

[ref11] 11. Tavares ALP, Garcia EL, Kuhn K, Woods CM, Williams T, et al. (2012) Ectodermal-derived Endothelin1 is required for patterning the distal and intermediate domains of the mouse mandibular arch. Developmental Biology 371: 47–56.
View Article
Google Scholar

[32] View Article

[33] Google Scholar

[ref12] 12. Miller CT, Yelon D, Stainier DY, Kimmel CB (2003) Two endothelin 1 effectors, hand2 and bapx1, pattern ventral pharyngeal cartilage and the jaw joint. Development 130: 1353–1365.
View Article
Google Scholar

[35] View Article

[36] Google Scholar

[ref13] 13. Barron F, Woods C, Kuhn K, Bishop J, Howard MJ, et al. (2011) Downregulation of Dlx5 and Dlx6 expression by Hand2 is essential for initiation of tongue morphogenesis. Development 138: 2249–2259.
View Article
Google Scholar

[38] View Article

[39] Google Scholar

[ref14] 14. Zuniga E, Stellabotte F, Crump JG (2010) Jagged-Notch signaling ensures dorsal skeletal identity in the vertebrate face. Development 137: 1843–1852.
View Article
Google Scholar

[41] View Article

[42] Google Scholar

[ref15] 15. Zuniga E, Rippen M, Alexander C, Schilling TF, Crump JG (2011) Gremlin 2 regulates distinct roles of BMP and Endothelin 1 signaling in dorsoventral patterning of the facial skeleton. Development 138: 5147–5156.
View Article
Google Scholar

[44] View Article

[45] Google Scholar

[ref16] 16. Alexander C, Zuniga E, Blitz IL, Wada N, Le Pabic P, et al. (2011) Combinatorial roles for BMPs and Endothelin 1 in patterning the dorsal-ventral axis of the craniofacial skeleton. Development 138: 5135–5146.
View Article
Google Scholar

[47] View Article

[48] Google Scholar

[ref17] 17. Kurihara Y, Kurihara H, Suzuki H, Kodama T, Maemura K, et al. (1994) Elevated blood pressure and craniofacial abnormalities in mice deficient in endothelin-1. Nature 368: 703–710.
View Article
Google Scholar

[50] View Article

[51] Google Scholar

[ref18] 18. Clouthier DE, Hosoda K, Richardson JA, Williams SC, Yanagisawa H, et al. (1998) Cranial and cardiac neural crest defects in endothelin-A receptor-deficient mice. Development 125: 813–824.
View Article
Google Scholar

[53] View Article

[54] Google Scholar

[ref19] 19. Yanagisawa H, Yanagisawa M, Kapur RP, Richardson JA, Williams SC, et al. (1998) Dual genetic pathways of endothelin-mediated intercellular signaling revealed by targeted disruption of endothelin converting enzyme-1 gene. Development 125: 825–836.
View Article
Google Scholar

[56] View Article

[57] Google Scholar

[ref20] 20. Abe M, Ruest LB, Clouthier DE (2007) Fate of cranial neural crest cells during craniofacial development in endothelin-A receptor-deficient mice. Int J Dev Biol 51: 97–105.
View Article
Google Scholar

[59] View Article

[60] Google Scholar

[ref21] 21. Kempf H, Linares C, Corvol P, Gasc JM (1998) Pharmacological inactivation of the endothelin type A receptor in the early chick embryo: a model of mispatterning of the branchial arch derivatives. Development 125: 4931–4941.
View Article
Google Scholar

[62] View Article

[63] Google Scholar

[ref22] 22. Srivastava D (1997) Regulation of cardiac mesodermal and neural crest development by the bHLH transcription factor, dHAND (vol 16, pg 154, 1997). Nature Genetics 16: 410–410.
View Article
Google Scholar

[65] View Article

[66] Google Scholar

[ref23] 23. Walker MB, Miller CT, Coffin Talbot J, Stock DW, Kimmel CB (2006) Zebrafish furin mutants reveal intricacies in regulating Endothelin1 signaling in craniofacial patterning. Dev Biol 295: 194–205.
View Article
Google Scholar

[68] View Article

[69] Google Scholar

[ref24] 24. Nichols JT, Pan L, Moens CB, Kimmel CB (2013) barx1 represses joints and promotes cartilage in the craniofacial skeleton. Development In Press.

[ref25] 25. Klingenberg CP (2009) Morphometric integration and modularity in configurations of landmarks: tools for evaluating a priori hypotheses. Evolution & Development 11: 405–421.
View Article
Google Scholar

[72] View Article

[73] Google Scholar

[ref26] 26. Klingenberg CP (2011) MorphoJ: an integrated software package for geometric morphometrics. Molecular Ecology Resources 11: 353–357.
View Article
Google Scholar

[75] View Article

[76] Google Scholar

[ref27] 27. Nair S, Li W, Cornell R, Schilling TF (2007) Requirements for Endothelin type-A receptors and Endothelin-1 signaling in the facial ectoderm for the patterning of skeletogenic neural crest cells in zebrafish. Development 134: 335–345.
View Article
Google Scholar

[78] View Article

[79] Google Scholar

[ref28] 28. Aiyer AR, Honarpour N, Herz J, Srivastava D (2005) Loss of Apaf-1 leads to partial rescue of the HAND2-null phenotype. Developmental Biology 278: 155–162.
View Article
Google Scholar

[81] View Article

[82] Google Scholar

[ref29] 29. Bonano M, Tribulo C, De Calisto J, Marchant L, Sanchez SS, et al. (2008) A new role for the Endothelin-1/Endothelin-A receptor signaling during early neural crest specification. Developmental Biology 323: 114–129.
View Article
Google Scholar

[84] View Article

[85] Google Scholar

[ref30] 30. Bagnato A, Tecce R, DiCastro V, Catt KJ (1997) Activation of mitogenic signaling by endothelin 1 in ovarian carcinoma cells. Cancer Research 57: 1306–1311.
View Article
Google Scholar

[87] View Article

[88] Google Scholar

[ref31] 31. Del Bufalo D, Di Castro V, Birocco A, Salani D, Rosano L, et al. (2002) Endothelin-1 acts as a survival factor in ovarian carcinoma cells. Clinical Science 103: 302S–305S.
View Article
Google Scholar

[90] View Article

[91] Google Scholar

[ref32] 32. Del Bufalo D, Di Castro V, Biroccio A, Varmi M, Salani D, et al. (2002) Endothelin-1 protects ovarian carcinoma cells against paclitaxel-induced apoptosis: Requirement for Akt activation. Molecular Pharmacology 61: 524–532.
View Article
Google Scholar

[93] View Article

[94] Google Scholar

[ref33] 33. Avery L, Wasserman S (1992) Ordering gene function: the interpretation of epistasis in regulatory hierarchies. Trends Genet 8: 312–316.
View Article
Google Scholar

[96] View Article

[97] Google Scholar

[ref34] 34. Westerfield M (1993) The zebrafish book: A guide for the laboratory use of zebrafish (Brachydanio rerio).

[ref35] 35. Kimmel CB, Ballard WW, Kimmel SR, Ullmann B, Schilling TF (1995) Stages of embryonic development of the zebrafish. Dev Dyn 203: 253–310.
View Article
Google Scholar

[100] View Article

[101] Google Scholar

[ref36] 36. Yelon D, Ticho B, Halpern ME, Ruvinsky I, Ho RK, et al. (2000) The bHLH transcription factor hand2 plays parallel roles in zebrafish heart and pectoral fin development. Development 127: 2573–2582.
View Article
Google Scholar

[103] View Article

[104] Google Scholar

[ref37] 37. Lawson ND, Weinstein BM (2002) In vivo imaging of embryonic vascular development using transgenic zebrafish. Dev Biol 248: 307–318.
View Article
Google Scholar

[106] View Article

[107] Google Scholar

[ref38] 38. Berghmans S, Murphey RD, Wienholds E, Neuberg D, Kutok JL, et al. (2005) tp53 mutant zebrafish develop malignant peripheral nerve sheath tumors. Proceedings of the National Academy of Sciences of the United States of America 102: 407–412.
View Article
Google Scholar

[109] View Article

[110] Google Scholar

[ref39] 39. Walker MB, Kimmel CB (2007) A two-color acid-free cartilage and bone stain for zebrafish larvae. Biotech Histochem 82: 23–28.
View Article
Google Scholar

[112] View Article

[113] Google Scholar

[ref40] 40. Eames BF, Yan YL, Swartz ME, Levic DS, Knapik EW, et al. (2011) Mutations in fam20b and xylt1 Reveal That Cartilage Matrix Controls Timing of Endochondral Ossification by Inhibiting Chondrocyte Maturation. Plos Genetics 7.

[ref41] 41. Crump JG, Swartz ME, Kimmel CB (2004) An integrin-dependent role of pouch endoderm in hyoid cartilage development. PLoS biology 2: E244.
View Article
Google Scholar

[116] View Article

[117] Google Scholar

[ref42] 42. Huycke TR, Eames BF, Kimmel CB (2012) Hedgehog-dependent proliferation drives modular growth during morphogenesis of a dermal bone. Development 139: 2371–2380.
View Article
Google Scholar

[119] View Article

[120] Google Scholar

[ref43] 43. Rohlf FJ (2005) tps Dig version 2.04. Stony Brook: Department of Ecology and Evolution, State University of New York.

Figures

Abstract

Introduction

Results

Epistasis Analysis of Larval Cartilage Phenotypes: an edn1–hand2 Genetic Pathway

A Novel Interaction between edn1 and hand2 in the Embryonic Pharyngeal Arches

The Pharyngeal arch DV Extension Phenotypes are likely due to Changes in arch Size

edn1 and hand2 Interact to Control Cell Proliferation in the Ventral Pharyngeal Arches

hand2 Regulates Anterior Extension in the Ventral First arch in an edn1-independent Manner

Discussion

hand2 as a Negative Regulator of edn1-dependent Cell Proliferation

How does Control of Early Pharyngeal arch Phenotype Relate to the Later Cartilage Phenotype?

hand2 Negatively Regulates edn1-independent Morphogenetic Movement

Materials and Methods

Fish Stocks and Maintenance

Skeletal Staining and Morphometric Analysis

Microscopy

Geometric Morphometric and Volume Analyses

Cell Proliferation Assay

Cell Death Assay

Supporting Information

Figure S1.

Figure S2.

Table S1.

Movie S1.

Acknowledgments

Author Contributions

References