Planarians can regenerate a whole animal from only a small piece of their body, and have become an important model for stem cell biology. To identify regenerative processes dependent on Wnt growth factors in the planarian Schmidtea mediterranea (Smed), we analyzed RNAi phenotypes of Evi, a transmembrane protein specifically required for the secretion of Wnt ligands. We show that, during regeneration, Smed-evi loss-of-function prevents posterior identity, leading to two-headed planarians that resemble Smed-catenin1 RNAi animals. In addition, we observe regeneration defects of the nervous system that are not found after Smed-catenin1 RNAi. By systematic knockdown of all putative Smed Wnts in regenerating planarians, we identify Smed-WntP-1 and Smed-Wnt11-2 as the putative posterior organizers, and demonstrate that Smed-Wnt5 is a regulator of neuronal organization and growth. Thus, our study provides evidence that planarian Wnts are major regulators of regeneration, and that they signal through β-catenin-dependent and-independent pathways.

Keywords:
Anteroposterior axis, Brain patterning, Evi/Wls, Planarians, Regeneration, Wnt signaling

Planarians have a nearly unlimited capability of renewing lost body structures (reviewed by Saló,2006). Candidates for providing positional information during planarian regeneration are gradient-forming growth factors, such as Wnts. Wnts are secreted glycoproteins that behave as major organizers during embryonic development in various metazoan organisms (reviewed by Logan and Nusse, 2004). Canonical Wnt signaling is transduced through β-catenin, and mediates developmental processes, including axis specification (reviewed by Grigoryan et al., 2008). Some Wnts, such as mammalian Wnt5 (Slusarski et al., 1997), can signal through β-catenin-independent mechanisms, and control processes, such as cell polarity and directional movement (Witze et al.,2008).

Recently, β-catenin has been demonstrated to be essential in the establishment of anteroposterior (AP) identity during regeneration of the planarian species Schmidtea mediterranea(Gurley et al., 2008; Iglesias et al., 2008; Petersen and Reddien,2008). Smed-β-catenin1 silencing leads to a loss of posterior identity and complete anteriorization (`radial-like hypercephalyzed'planarians) (Iglesias et al.,2008). However, although these studies suggest that Wnt proteins might be essential organizers of regeneration in planarians, direct evidence is missing.

Wnt secretion requires the transmembrane protein Evenness interrupted [Evi;also known as Wntless (Wls) and Sprinter](Bänziger et al., 2006; Bartscherer et al., 2006; Goodman et al., 2006). In Drosophila and Caenorhabditis elegans, Wnts are not secreted in the absence of Evi, leading to a loss of Wnt signaling in the surrounding tissue. Owing to the lack of non-canonical phenotypes in evi mutant flies (Bartscherer et al.,2006), it is currently not known whether Evi also controlsβ-catenin-independent Wnt signaling.

Here, we report the effect of RNAi-mediated silencing of Smed-evi and all putative S. mediterranea Wnt genes during planarian regeneration. We show that, like Smed-β-catenin1,Smed-evi, as well as Smed-wnt11-2 and Smed-wntP-1, are required for posterior identity in regenerating animals. In addition, we demonstrate that Smed-evi RNAi causes the sameβ-catenin-independent defects as does Smed-wnt5loss-of-function, suggesting that Smed-Wnt5 is a non-canonical Wnt that requires Smed-Evi for its secretion, and which acts to control neuronal growth during regeneration of the planarian nervous system.

Animals

The planarians used belong to an asexual race of S. mediterranea,and were maintained as described elsewhere(Molina et al., 2007).

Identification and cloning of S. mediterranea genes

Smed-evi and the nine Smed-Wnt genes were identified from the S. mediterranea genomic database(http://genome.wustl.edu/)through a BLAST search(http://ncbi.nlm.nih.gov). The full-length transcripts of the incomplete genes were amplified by rapid amplification of cDNA ends (RACE) using the Invitrogen GeneRacer Kit(Invitrogen).

Accession numbers

Smed-evi, FJ463748; Smed-wnt5, FJ463749; Smed-wntA, FJ463750; Smed-wnt11-2, FJ463751; Smed-wntP-4, FJ463752.

RNAi silencing

dsRNA microinjection was performed as described elsewhere(Sánchez-Alvarado and Newmark,1999). dsRNAs were synthesized as described(Boutros et al., 2004). Primer details are available upon request. Control animals were injected with water. Injected planarians were amputated pre- and post-pharyngeally, and the head-,trunk-, and tail-pieces were allowed to regenerate for the times indicated.

Whole-mount in situ hybridization

Whole-mount in situ hybridization was carried out as described previously(Nogi and Levin, 2005; Umesono et al., 1999). Digoxigenin-labelled riboprobes were synthesized using an in vitro transcription kit (Roche) (Iglesias et al., 2008). Primer details are available upon request.

Whole-mount immunostaining

Immunostaining was carried out as described previously(Cebrià and Newmark,2005). Antibodies used were: anti-Arrestin(Sakai et al., 2000) at a 1:15,000 dilution, and anti-Synapsin (anti-SYNORF1, Developmental Studies Hybridoma Bank) at 1:25.

An Evi homolog is expressed in S. mediterranea

We found a single evi gene in the genome of S. mediterranea (Fig. 1A; see also Fig. S1 in the supplementary material). Smed-evi mRNA mainly localized to the nervous system, the brain/cephalic ganglia (CG) and the ventral nerve cords (VNCs), as well as to the pharynx, and to the mouth. In addition, it was expressed in discrete cells of the posterior parenchyma(Fig. 1B).

To analyze the expression of Smed-evi in regenerating animals, we dissected heads and tails from the trunk parts of the animals and followed their regeneration. Smed-evi was expressed in the regenerating nervous system and upregulated in the pharynx primordia, as well as in the tips of posterior wounds (blastemas; Fig. 1C), suggesting that Smed-evi might be especially important for posterior regeneration. As Evi is required for the secretion of Wnts, the Smed-evi expression pattern might indicate sites of Wnt production and release in planarians.

Smed-evi is required for posterior identity

To reveal Wnt-dependent processes in planarian regeneration, we depleted Smed-evi by RNAi, and dissected heads and tails from the trunk parts of the animals. Within 25 days of regeneration, all head fragments developed an ectopic posterior head with eyes and a brain(Fig. 2A,B). In addition, the expression of the central-posterior Hox gene Smed-hoxD was lost(Fig. 2C). These results indicate that, in the absence of Smed-evi, posterior fate is suppressed to the gain of anterior structures.

We obtained similar results for evi RNAi trunk fragments, as most of them developed an ectopic posterior head(Fig. 2D,E). In all animals,the anterior head showed several ectopic eyes. Both, anterior and posterior eyes differentiated laterally along the anteroposterior axis and were connected by their visual axons. In most cases, they did not cross the commissure and the optic quiasm was not formed(Fig. 2D). In ∼50% of the Smed-evi RNAi trunks, the posterior head dissociated spontaneously during regeneration, a process we refer to as `scission'. Tail pieces regenerated a head with ectopic eyes (for Smed-evi RNAi phenotypes,see Fig. S2 in the supplementary material).

The role of planarian Evi in AP polarity, but not in dorsoventral (DV)polarity (see Fig. S3 in the supplementary material), is consistent with the recently described Smed-β-catenin1 RNAi phenotype. Smed-β-catenin1 RNAi causes a loss of AP polarity and complete anteriorization of regenerating planarians(Gurley et al., 2008; Iglesias et al., 2008; Petersen and Reddien, 2008)(Fig. 2F). However, we never observed full anteriorization after Smed-evi knockdown, which might be due to inefficient knockdown of Smed-evi, or to a stronger blockage of signaling after the loss of Smed-β-catenin1.

Together our results suggest that Smed-Evi is required for the release of Wnts that act through a β-catenin-dependent pathway to organize AP axis polarity during planarian regeneration.

Smed-evi is required for neuronal growth regulation during regeneration

To analyze the brains of Smed-evi RNAi animals in more detail, we tested head fragments for Synapsin expression(Fig. 2G-J). In wild-type animals the CG were located dorsally above the VNCs and extended as a pair into the regenerating tail (Fig. 2G; see Movie 1 in the supplementary material). However, in the posterior head of Smed-evi RNAi animals, both CG grew laterally along the VNCs. Confocal sections revealed that the posterior part of the CG projected into the ventral region (Fig. 2G′; see Movie 2 in the supplementary material). We refer to this phenotype as `deflected-brain phenotype'. Even though Smed-β-catenin1 knockdown also resulted in the formation of a posterior brain, the ectopic CG never appeared deflected from the VNCs(Fig. 2H).

Fig. 1.
An Evi homolog is expressed in planarians. (A) Human, fly and planarian Evi proteins. Protein sizes and sequence identities are indicated. Putative transmembrane domains are blue. (B,C) Whole-mount in situ expression analysis of evi mRNA in Schmidtea mediterranea. In intact animals, Smed-evi mRNA is expressed in the cephalic ganglia (CG), the ventral nerve cords (VNCs), the mouth, the pharynx, and cells of the posterior parenchyma (B). During regeneration (C), Smed-evi is expressed in the regenerating nervous system, and is upregulated in the pharynx and in posterior blastemas (arrows). Shown are head, trunk and tail fragments six days after dissection. Anterior is left,posterior is right. Scale bar: 500 μm.
View largeDownload slide

An Evi homolog is expressed in planarians. (A) Human, fly and planarian Evi proteins. Protein sizes and sequence identities are indicated. Putative transmembrane domains are blue. (B,C) Whole-mount in situ expression analysis of evi mRNA in Schmidtea mediterranea. In intact animals, Smed-evi mRNA is expressed in the cephalic ganglia (CG), the ventral nerve cords (VNCs), the mouth, the pharynx, and cells of the posterior parenchyma (B). During regeneration (C), Smed-evi is expressed in the regenerating nervous system, and is upregulated in the pharynx and in posterior blastemas (arrows). Shown are head, trunk and tail fragments six days after dissection. Anterior is left,posterior is right. Scale bar: 500 μm.

Fig. 1.
An Evi homolog is expressed in planarians. (A) Human, fly and planarian Evi proteins. Protein sizes and sequence identities are indicated. Putative transmembrane domains are blue. (B,C) Whole-mount in situ expression analysis of evi mRNA in Schmidtea mediterranea. In intact animals, Smed-evi mRNA is expressed in the cephalic ganglia (CG), the ventral nerve cords (VNCs), the mouth, the pharynx, and cells of the posterior parenchyma (B). During regeneration (C), Smed-evi is expressed in the regenerating nervous system, and is upregulated in the pharynx and in posterior blastemas (arrows). Shown are head, trunk and tail fragments six days after dissection. Anterior is left,posterior is right. Scale bar: 500 μm.
View largeDownload slide

An Evi homolog is expressed in planarians. (A) Human, fly and planarian Evi proteins. Protein sizes and sequence identities are indicated. Putative transmembrane domains are blue. (B,C) Whole-mount in situ expression analysis of evi mRNA in Schmidtea mediterranea. In intact animals, Smed-evi mRNA is expressed in the cephalic ganglia (CG), the ventral nerve cords (VNCs), the mouth, the pharynx, and cells of the posterior parenchyma (B). During regeneration (C), Smed-evi is expressed in the regenerating nervous system, and is upregulated in the pharynx and in posterior blastemas (arrows). Shown are head, trunk and tail fragments six days after dissection. Anterior is left,posterior is right. Scale bar: 500 μm.

In bipolar regenerating trunk fragments, Synapsin expression showed the same deflected-brain phenotype. In addition, longitudinal neuronal tissue projected from posterior CG into the ventral half of the animal(Fig. 2I′; see Movie 4 in the supplementary material; a control trunk fragment is shown in Movie 3). We can only speculate whether these projections were new VNCs growing from posterior to anterior. As they grew laterally to the old VNCs, it is possible that old ones might repel new neuronal tissue, causing the lateral protrusions we observed in regenerating trunks (Fig. 2D,I′). Consistent with the absence of any optical chiasm,Synapsin staining revealed that the commissure was lost in anterior and posterior brains. We also observed a disconnection between the old and the new VNCs. Smed-β-catenin1 RNAi animals showed neither a deflection nor any disconnections of the nervous tissue(Fig. 2J). Thus, we propose that Smed-Evi is required for the release of a Wnt protein that does not signal through β-catenin, and which restricts and defines the position of neuronal tissue during planarian regeneration.

Fig. 2.
Smed-evi RNAi phenotypes. (A-E) Smed-eviRNAi results in anteriorized planarians. Images of live animals(A,D,D′), and animals stained for visual Arrestin (A′,D″). Note the formation of a posterior head, indicated by white arrows pointing towards ectopic eyes. Orange arrows indicate ectopic lateral protrusions (see also I′). Loss of the optical chiasm is indicated by the white arrowhead in D″. (B,E) Whole-mount in situ hybridization against Smed-glutamate receptor (gluR) mRNA shows the formation of an ectopic brain instead of a tail in Smed-eviRNAi animals (arrow). (C) Whole-mount in situ hybridization against Smed-hoxD mRNA indicates the loss of posterior and medial identities after Smed-evi RNAi. (F) RNAi against Smed-β-catenin1 leads to fully anteriorized planarians.(G,G′,I,I′) Smed-evi RNAi results in growth and patterning defects of the regenerating nervous system. The nervous system was labeled with an anti-Synapsin antibody (green). The position of Arrestin-positive eyes is indicated in red (pseudocolor). In control head fragments (G) CG (red arrows) are located dorsally above the VNCs (blue arrows). After Smed-evi RNAi (G′), the posterior CG are detected in dorsal and ventral sections, laterally to the VNCs(deflected-brain phenotype). (I,I′) Regenerating trunk fragments. After Smed-evi RNAi, both anterior and posterior nervous tissue show the deflected-brain phenotype. CG,red arrows; VNCs, blue arrows, putative VNCs projected from posterior CG, purple arrows; disconnections between the old and the new nervous tissue, white arrows. (H,J) Synapsin expression in regenerating head and trunk fragments after Smed-β-catenin1RNAi. Regenerating head and trunk animals correspond to 20 and 25-30 days of regeneration. Images are z-projections of several confocal sections. Dorsal and ventral images are single sections. Anterior is left, posterior is right.
View largeDownload slide

Smed-evi RNAi phenotypes. (A-E) Smed-eviRNAi results in anteriorized planarians. Images of live animals(A,D,D′), and animals stained for visual Arrestin (A′,D″). Note the formation of a posterior head, indicated by white arrows pointing towards ectopic eyes. Orange arrows indicate ectopic lateral protrusions (see also I′). Loss of the optical chiasm is indicated by the white arrowhead in D″. (B,E) Whole-mount in situ hybridization against Smed-glutamate receptor (gluR) mRNA shows the formation of an ectopic brain instead of a tail in Smed-eviRNAi animals (arrow). (C) Whole-mount in situ hybridization against Smed-hoxD mRNA indicates the loss of posterior and medial identities after Smed-evi RNAi. (F) RNAi against Smed-β-catenin1 leads to fully anteriorized planarians.(G,G′,I,I′) Smed-evi RNAi results in growth and patterning defects of the regenerating nervous system. The nervous system was labeled with an anti-Synapsin antibody (green). The position of Arrestin-positive eyes is indicated in red (pseudocolor). In control head fragments (G) CG (red arrows) are located dorsally above the VNCs (blue arrows). After Smed-evi RNAi (G′), the posterior CG are detected in dorsal and ventral sections, laterally to the VNCs(deflected-brain phenotype). (I,I′) Regenerating trunk fragments. After Smed-evi RNAi, both anterior and posterior nervous tissue show the deflected-brain phenotype. CG,red arrows; VNCs, blue arrows, putative VNCs projected from posterior CG, purple arrows; disconnections between the old and the new nervous tissue, white arrows. (H,J) Synapsin expression in regenerating head and trunk fragments after Smed-β-catenin1RNAi. Regenerating head and trunk animals correspond to 20 and 25-30 days of regeneration. Images are z-projections of several confocal sections. Dorsal and ventral images are single sections. Anterior is left, posterior is right.

Fig. 2.
Smed-evi RNAi phenotypes. (A-E) Smed-eviRNAi results in anteriorized planarians. Images of live animals(A,D,D′), and animals stained for visual Arrestin (A′,D″). Note the formation of a posterior head, indicated by white arrows pointing towards ectopic eyes. Orange arrows indicate ectopic lateral protrusions (see also I′). Loss of the optical chiasm is indicated by the white arrowhead in D″. (B,E) Whole-mount in situ hybridization against Smed-glutamate receptor (gluR) mRNA shows the formation of an ectopic brain instead of a tail in Smed-eviRNAi animals (arrow). (C) Whole-mount in situ hybridization against Smed-hoxD mRNA indicates the loss of posterior and medial identities after Smed-evi RNAi. (F) RNAi against Smed-β-catenin1 leads to fully anteriorized planarians.(G,G′,I,I′) Smed-evi RNAi results in growth and patterning defects of the regenerating nervous system. The nervous system was labeled with an anti-Synapsin antibody (green). The position of Arrestin-positive eyes is indicated in red (pseudocolor). In control head fragments (G) CG (red arrows) are located dorsally above the VNCs (blue arrows). After Smed-evi RNAi (G′), the posterior CG are detected in dorsal and ventral sections, laterally to the VNCs(deflected-brain phenotype). (I,I′) Regenerating trunk fragments. After Smed-evi RNAi, both anterior and posterior nervous tissue show the deflected-brain phenotype. CG,red arrows; VNCs, blue arrows, putative VNCs projected from posterior CG, purple arrows; disconnections between the old and the new nervous tissue, white arrows. (H,J) Synapsin expression in regenerating head and trunk fragments after Smed-β-catenin1RNAi. Regenerating head and trunk animals correspond to 20 and 25-30 days of regeneration. Images are z-projections of several confocal sections. Dorsal and ventral images are single sections. Anterior is left, posterior is right.
View largeDownload slide

Smed-evi RNAi phenotypes. (A-E) Smed-eviRNAi results in anteriorized planarians. Images of live animals(A,D,D′), and animals stained for visual Arrestin (A′,D″). Note the formation of a posterior head, indicated by white arrows pointing towards ectopic eyes. Orange arrows indicate ectopic lateral protrusions (see also I′). Loss of the optical chiasm is indicated by the white arrowhead in D″. (B,E) Whole-mount in situ hybridization against Smed-glutamate receptor (gluR) mRNA shows the formation of an ectopic brain instead of a tail in Smed-eviRNAi animals (arrow). (C) Whole-mount in situ hybridization against Smed-hoxD mRNA indicates the loss of posterior and medial identities after Smed-evi RNAi. (F) RNAi against Smed-β-catenin1 leads to fully anteriorized planarians.(G,G′,I,I′) Smed-evi RNAi results in growth and patterning defects of the regenerating nervous system. The nervous system was labeled with an anti-Synapsin antibody (green). The position of Arrestin-positive eyes is indicated in red (pseudocolor). In control head fragments (G) CG (red arrows) are located dorsally above the VNCs (blue arrows). After Smed-evi RNAi (G′), the posterior CG are detected in dorsal and ventral sections, laterally to the VNCs(deflected-brain phenotype). (I,I′) Regenerating trunk fragments. After Smed-evi RNAi, both anterior and posterior nervous tissue show the deflected-brain phenotype. CG,red arrows; VNCs, blue arrows, putative VNCs projected from posterior CG, purple arrows; disconnections between the old and the new nervous tissue, white arrows. (H,J) Synapsin expression in regenerating head and trunk fragments after Smed-β-catenin1RNAi. Regenerating head and trunk animals correspond to 20 and 25-30 days of regeneration. Images are z-projections of several confocal sections. Dorsal and ventral images are single sections. Anterior is left, posterior is right.

Wnt genes in the S. mediterranea genome

To identify all putative Wnt genes in S. mediterranea, we searched the genome for sequences homologous to Wnts from several species. We identified nine Wnt genes: Smed-wntP-1, Smed-wntP-2, Smed-wntP-3,Smed-wnt11-1 and Smed-wnt2-1, have been recently reported(Petersen and Reddien, 2008); Smed-wntA and Smed-wnt5 encode proteins homologous to Wnts from other planarian species (Kobayashi et al., 2007; Marsal et al.,2003); and Smed-wnt11-2 and Smed-wntP-4 have not been described before. Phylogenetic analysis demonstrates that Smed-Wnt5,Smed-Wnt11-1/2 and Smed-Wnt2-1 can be assigned to established Wnt subfamilies. However, the other planarian Wnts appear as internal duplications in this phylum, and cannot be classified with high certainty (see Fig. S4 in the supplementary material).

Posterior identity requires Smed-wntP-1 and Smed-wnt11-2

Next, we set out to identify the Wnts responsible for the specification of posterior structures during regeneration. In situ hybridization experiments showed that Smed-wnt11-2, as well as Smed-wntP-1(Petersen and Reddien, 2008),was expressed in discrete cells along the most posterior midline of the S. mediterranea body (Fig. 3A,B). In regenerating animals, Smed-wnt11-2 and Smed-wntP-1 mRNA levels were upregulated in discrete cells of the posterior blastemas, indicating an important role in the control of posterior identity (Fig. 3C,D).

We tested whether posterior regeneration was affected by Smed-wnt11-2 and Smed-wntP-1 RNAi. Silencing of either mRNA led to a `tailless' morphology, which was characterized by a shorter and more rounded posterior end, in which VNCs terminated shortly behind the pharynx(Fig. 3F,G). Furthermore,∼10% of regenerating trunks, and more than half of all regenerating head fragments of Smed-wntP-1 RNAi animals resulted in two-headed planarians (Fig. 3G), a phenotype that was not enhanced by the simultaneous knockdown of wnt11-2 (not shown). As Smed-β-catenin1 RNAi also causes anteriorization of planarians (Fig. 2), Smed-Wnt11-2 and Smed-WntP-1 are likely to signal throughβ-catenin to permit posterior fate during regeneration.

Fig. 3.
Smed-wnt11-2 and Smed-wntP-1 are required for posterior identity during planarian regeneration. (A-D) Whole-mount in situ hybridization analysis of Smed-wnt11-2 and Smed-wntP-1 mRNAs (arrows) in intact (A,B) and regenerating animals at day 4 of regeneration (C,D). (F,G) RNAi against Smed-wnt11-2 and Smed-wntP-1 leads to a `tailless' phenotype(red arrows, compare with control in E). In some animals (see quantification in G″), Smed-wntP-1 RNAi causes the generation of ectopic posterior heads (white arrows in G). Shown are images of live regenerating trunk fragments (E-G), and confocal z-projections of trunk fragments stained with anti-Synapsin (E′-G′), at day 20 of regeneration.
View largeDownload slide

Smed-wnt11-2 and Smed-wntP-1 are required for posterior identity during planarian regeneration. (A-D) Whole-mount in situ hybridization analysis of Smed-wnt11-2 and Smed-wntP-1 mRNAs (arrows) in intact (A,B) and regenerating animals at day 4 of regeneration (C,D). (F,G) RNAi against Smed-wnt11-2 and Smed-wntP-1 leads to a `tailless' phenotype(red arrows, compare with control in E). In some animals (see quantification in G″), Smed-wntP-1 RNAi causes the generation of ectopic posterior heads (white arrows in G). Shown are images of live regenerating trunk fragments (E-G), and confocal z-projections of trunk fragments stained with anti-Synapsin (E′-G′), at day 20 of regeneration.

Fig. 3.
Smed-wnt11-2 and Smed-wntP-1 are required for posterior identity during planarian regeneration. (A-D) Whole-mount in situ hybridization analysis of Smed-wnt11-2 and Smed-wntP-1 mRNAs (arrows) in intact (A,B) and regenerating animals at day 4 of regeneration (C,D). (F,G) RNAi against Smed-wnt11-2 and Smed-wntP-1 leads to a `tailless' phenotype(red arrows, compare with control in E). In some animals (see quantification in G″), Smed-wntP-1 RNAi causes the generation of ectopic posterior heads (white arrows in G). Shown are images of live regenerating trunk fragments (E-G), and confocal z-projections of trunk fragments stained with anti-Synapsin (E′-G′), at day 20 of regeneration.
View largeDownload slide

Smed-wnt11-2 and Smed-wntP-1 are required for posterior identity during planarian regeneration. (A-D) Whole-mount in situ hybridization analysis of Smed-wnt11-2 and Smed-wntP-1 mRNAs (arrows) in intact (A,B) and regenerating animals at day 4 of regeneration (C,D). (F,G) RNAi against Smed-wnt11-2 and Smed-wntP-1 leads to a `tailless' phenotype(red arrows, compare with control in E). In some animals (see quantification in G″), Smed-wntP-1 RNAi causes the generation of ectopic posterior heads (white arrows in G). Shown are images of live regenerating trunk fragments (E-G), and confocal z-projections of trunk fragments stained with anti-Synapsin (E′-G′), at day 20 of regeneration.

Smed-Wnt5 controls neuronal growth and patterning during regeneration

To identify Wnt proteins responsible for the deflected-brain phenotype of Smed-evi RNAi animals, we silenced all remaining S. mediterranea Wnt transcripts. Smed-wnt2-1, Smed-wntP-3 and Smed-wntP-4 had no obvious phenotype, possibly owing to inefficient knockdown. Consistent with the phenotype after DjwntA silencing in the planarian species Dugesia japonica(Kobayashi et al., 2007), we detected an abnormal elongation of the new brain and visual axons in Smed-wntA RNAi animals (see Fig. S5 in the supplementary material).

In Smed-wnt5 RNAi animals, we discovered a deflection and ventral expansion of the regenerating CG (Fig. 4D; see also Movie 5 in the supplementary material). In the regenerating tail, new Synapsin-positive tissue appeared, which was thicker than, and appeared disconnected from, the old nervous tissue(Fig. 4D). Expression analysis of Smed-glutamate receptor (gluR) mRNA showed that the new posterior neuronal tissue was not of brain identity(Fig. 4E), suggesting that it was new VNCs that grew deflected from the old ones. These phenotypes were similar to those observed after Smed-evi silencing(Fig. 2I; see also Movie 5 in the supplementary material).

Consistent with this, we found that Smed-wnt5 mRNA localized mainly to distinct cells along the CG and VNCs, and was upregulated in the regenerating nervous system and the blastemas(Fig. 4B). Together, our data suggest that Smed-Evi restricts and coordinates the growth of regenerating neuronal tissue by regulating the secretion of Smed-Wnt5.

Concluding remarks

Our study reveals several regenerative processes that are regulated by Wnts in planarians (for a summary, see Table S1 in the supplementary material). Using Smed-evi RNAi to block Wnt secretion, we identify AP axis polarity and neuronal growth as being Wnt-regulated processes. Specifically,we identify Smed-wntP-1 and Smed-wnt11-2 as being the secreted molecules responsible for AP axis polarity. Consistent with the role of Wnts as morphogens (reviewed by Bartscherer and Boutros, 2008),Smed-WntP-1 and Smed-Wnt11-2 might activate posterior fate, from their site of production in the tail (Fig. 3), along the AP body axis. As posterior identity also depends on Smed-β-catenin1, we propose that Smed-WntP-1 and Smed-Wnt11-2 signal through β-catenin to permit posterior fate during regeneration.

Furthermore, we show that knockdown of Smed-wnt5 results in a deflected-brain phenotype. Our data are consistent with the reported role of Wnt5 in axonal growth in several organisms(Yoshikawa et al., 2003; Fradkin et al., 2004; Zhang et al., 2007). Smed-Wnt5 belongs to the Wnt5 family (see Fig. S4 in the supplementary material), which has been linked to non-canonical Wnt signal transduction(Wong et al., 1994; Olson and Papkoff, 1994; Shimizu et al., 1997) and seems to regulate cell motility rather than specification(Moon et al., 1993; Wallingford et al., 2001; Witze et al., 2008). As we did not observe any deflected-brain phenotype after Smed-β-catenin1RNAi, we suggest that Smed-Wnt5 signals through a mechanism that isβ-catenin independent.

In planarians, Evi function is therefore required for the secretion of Wnts that signal through β-catenin-dependent and -independent pathways(Fig. 4F). This suggests that Evi is an ancient factor that had been an important facilitator of Wnt secretion before Wnts functionally diverged. Even though the same Wnts might be able to signal through both canonical and non-canonical pathways, depending on the receptor context (reviewed by van Amerongen et al., 2008), we demonstrate that Wnts can have distinct canonical or non-canonical functions in planarians. The nature and constellation of planarian Wnt receptors remains the subject of future studies, and might help us to understand how cells translate Wnt signals into diverse cellular responses, both in planarians and in other organisms.

Fig. 4.
Smed-wnt5 regulates growth and patterning of the planarian regenerating nervous system. (A,B) In situ hybridization analysis of Smed-wnt5 mRNA in intact (A) and regenerating (B)animals. Smed-wnt5 is expressed in discrete cells along the VNCs and the CG (red arrows), as well as in cells in the periphery and along the DV boundary (blue arrows). It is upregulated in the regenerating CG of the anterior blastema (white arrows in B). (C,D) Control and Smed-wnt5 RNAi trunk fragments at day 20 of regeneration, stained with anti-Synapsin. Red arrows point to CG, blue arrows to VNCs. Note the deflection and expansion of regenerating nervous tissue in Smed-wnt5 RNAi animals. White arrows indicate the disconnection between old and new nervous tissue. Images are z-projections, dorsal and ventral views are single sections. (E) In situ hybridization analyis of gluRmRNA. No brain tissue is detected in the tail. (F) Summary of RNAi phenotypes of regenerating trunk fragments. Shown are dorsal and lateral views. Yellow indicates CG; green, VNCs. A, anterior; P, posterior; D, dorsal;V, ventral.
View largeDownload slide

Smed-wnt5 regulates growth and patterning of the planarian regenerating nervous system. (A,B) In situ hybridization analysis of Smed-wnt5 mRNA in intact (A) and regenerating (B)animals. Smed-wnt5 is expressed in discrete cells along the VNCs and the CG (red arrows), as well as in cells in the periphery and along the DV boundary (blue arrows). It is upregulated in the regenerating CG of the anterior blastema (white arrows in B). (C,D) Control and Smed-wnt5 RNAi trunk fragments at day 20 of regeneration, stained with anti-Synapsin. Red arrows point to CG, blue arrows to VNCs. Note the deflection and expansion of regenerating nervous tissue in Smed-wnt5 RNAi animals. White arrows indicate the disconnection between old and new nervous tissue. Images are z-projections, dorsal and ventral views are single sections. (E) In situ hybridization analyis of gluRmRNA. No brain tissue is detected in the tail. (F) Summary of RNAi phenotypes of regenerating trunk fragments. Shown are dorsal and lateral views. Yellow indicates CG; green, VNCs. A, anterior; P, posterior; D, dorsal;V, ventral.

Fig. 4.
Smed-wnt5 regulates growth and patterning of the planarian regenerating nervous system. (A,B) In situ hybridization analysis of Smed-wnt5 mRNA in intact (A) and regenerating (B)animals. Smed-wnt5 is expressed in discrete cells along the VNCs and the CG (red arrows), as well as in cells in the periphery and along the DV boundary (blue arrows). It is upregulated in the regenerating CG of the anterior blastema (white arrows in B). (C,D) Control and Smed-wnt5 RNAi trunk fragments at day 20 of regeneration, stained with anti-Synapsin. Red arrows point to CG, blue arrows to VNCs. Note the deflection and expansion of regenerating nervous tissue in Smed-wnt5 RNAi animals. White arrows indicate the disconnection between old and new nervous tissue. Images are z-projections, dorsal and ventral views are single sections. (E) In situ hybridization analyis of gluRmRNA. No brain tissue is detected in the tail. (F) Summary of RNAi phenotypes of regenerating trunk fragments. Shown are dorsal and lateral views. Yellow indicates CG; green, VNCs. A, anterior; P, posterior; D, dorsal;V, ventral.
View largeDownload slide

Smed-wnt5 regulates growth and patterning of the planarian regenerating nervous system. (A,B) In situ hybridization analysis of Smed-wnt5 mRNA in intact (A) and regenerating (B)animals. Smed-wnt5 is expressed in discrete cells along the VNCs and the CG (red arrows), as well as in cells in the periphery and along the DV boundary (blue arrows). It is upregulated in the regenerating CG of the anterior blastema (white arrows in B). (C,D) Control and Smed-wnt5 RNAi trunk fragments at day 20 of regeneration, stained with anti-Synapsin. Red arrows point to CG, blue arrows to VNCs. Note the deflection and expansion of regenerating nervous tissue in Smed-wnt5 RNAi animals. White arrows indicate the disconnection between old and new nervous tissue. Images are z-projections, dorsal and ventral views are single sections. (E) In situ hybridization analyis of gluRmRNA. No brain tissue is detected in the tail. (F) Summary of RNAi phenotypes of regenerating trunk fragments. Shown are dorsal and lateral views. Yellow indicates CG; green, VNCs. A, anterior; P, posterior; D, dorsal;V, ventral.

We thank F. Cebrià for helpful advice; M. Riutort for help with phylogenetic analysis of Wnt proteins; M. Carl and A. Ragab for comments on the manuscript; B. Lang and T. Horn for bioinformatics support; F. Cebrià and P. Newmark for providing Smed-gluR, septinand eye53 clones; H. Orii and K. Watanabe for providing anti-Arrestin. K.B. thanks M. Osborn and M. Schäfer for advice. This work was supported by a Marie Curie Excellence grant from the European Commission, the German Research Foundation and by the Ministerio de Ciencia e Innovación, Spain.

Supplementary material

van Amerongen, R., Mikels, A. and Nusse, R.(
2008
). Alternative wnt signaling is initiated by distinct receptors.
Sci. Signal.
1
,
re9
.
Bänziger, C., Soldini, D., Schütt, C., Zipperlen, P.,Hausmann, G. and Basler, K. (
2006
). Wntless, a conserved membrane protein dedicated to the secretion of Wnt proteins from signaling cells.
Cell
125
,
509
-522.
Bartscherer, K. and Boutros, M. (
2008
). Regulation of Wnt protein secretion and its role in gradient formation.
EMBO Rep.
9
,
977
-982.
Bartscherer, K., Pelte, N., Ingelfinger, D. and Boutros, M.(
2006
). Secretion of Wnt ligands requires Evi, a conserved transmembrane protein.
Cell
125
,
523
-533.
Boutros, M., Kiger, A. A., Armknecht, S., Kerr, K., Hild, M.,Koch, B., Haas, S. A., Paro, R. and Perrimon, N. (
2004
). Heidelberg Fly Array Consortium. Genome-wide RNAi analysis of growth and viability in Drosophila cells.
Science
303
,
832
-835.
Cebrià, F. and Newmark, P. A. (
2005
). Planarian homologs of netrin and netrin receptor are required for proper regeneration of the central nervous system and the maintenance of nervous system architecture.
Development
132
,
3691
-3703.
Fradkin, L. G., van Schie, M., Wouda, R. R., de Jong, A.,Kamphorst, J. T., Radjkoemar-Bansraj, M. and Noordermeer, J. N.(
2004
). The Drosophila Wnt5 protein mediates selective axon fasciculation in the embryonic central nervous system.
Dev. Biol.
272
,
362
-375.
Goodman, R. M., Thombre, S., Firtina, Z., Gray, D., Betts, D.,Roebuck, J., Spana, E. P. and Selva, E. M. (
2006
). Sprinter:a novel transmembrane protein required for Wg secretion and signaling.
Development
133
,
4901
-4911.
Grigoryan, T., Wend, P., Klaus, A. and Birchmeier, W.(
2008
). Deciphering the function of canonical Wnt signals in development and disease: conditional loss- and gain-of-function mutations ofβ-catenin in mice.
Genes Dev.
22
,
2308
-2341.
Gurley, K. A., Rink, J. C. and Sánchez Alvarado, A.(
2008
). β-catenin defines head versus tail identity during planarian regeneration and homeostasis.
Science
319
,
323
-327.
Iglesias, M., Gomez-Skarmeta, J. L., Saló, E. and Adell,T. (
2008
). Silencing of Smed-βcatenin1 generates radial-like hypercephalized planarians.
Development
135
,
1215
-1221.
Kobayashi, C., Saito, Y., Ogawa, K. and Agata, K.(
2007
). Wnt signaling is required for antero-posterior patterning of the planarian brain.
Dev. Biol.
306
,
714
-724.
Logan, C. Y. and Nusse, R. (
2004
). The Wnt signaling pathway in development and disease.
Annu. Rev. Cell Dev. Biol.
20
,
781
-810.
Marsal, M., Pineda, D. and Saló, E.(
2003
). Gtwnt-5 a member of the wnt family expressed in a subpopulation of the nervous system of the planarian Girardia tigrina.
Gene Expr. Patterns
3
,
489
-495.
Molina, M. D., Saló, E. and Cebrià, F.(
2007
). The BMP pathway is essential for re-specification and maintenance of the dorsoventral axis in regenerating and intact planarians.
Dev. Biol.
311
,
79
-94.
Moon, R. T., Campbell, R. M., Christian, J. L., McGrew, L. L.,Shih, J. and Fraser, S. (
1993
). Xwnt-5A: a maternal Wnt that affects morphogenetic movements after overexpression in embryos of Xenopus laevis.
Development
119
,
97
-111.
Nogi, N. and Levin, M. (
2005
). Characterization of innexin gene expression and functional roles of gap-junctional communication in planarian regeneration.
Dev. Biol.
287
,
314
-335.
Olson, D. J. and Papkoff, J. (
1994
). Regulated expression of Wnt family members during proliferation of C57mg mammary cells.
Cell Growth Differ.
5
,
197
-206.
Petersen, C. P. and Reddien, P. W. (
2008
). Smed-βcatenin-1 is required for anteroposterior blastema polarity in planarian regeneration.
Science
319
,
327
-330.
Sakai, F., Agata, K., Orii, H. and Watanabe, K.(
2000
). Organization and regeneration ability of spontaneous supernumerary eyes in planarians-Eye regeneration field and pathway selection by optic nerves.
Zool. Sci.
17
,
375
-381.
Saló, E. (
2006
). The power of regeneration and the stem-cell kingdom: freshwater planarians(Platyhelminthes).
BioEssays
28
,
546
-559.
Sánchez Alvarado, A. and Newmark, P.(
1999
). Double-stranded RNA specifically disrupts gene expression during planarian regeneration.
Proc. Natl. Acad. Sci. USA
96
,
5049
-5054.
Shimizu, H., Julius, M. A., Giarré, M., Zheng, Z., Brown,A. M. and Kitajewski, J. (
1997
).Transformation by Wnt family proteins correlates with regulation of β-catenin.
Cell Growth Differ.
8
,
1349
-1358.
Slusarski, D. C., Yang-Snyder, J., Busa, W. B. and Moon, R. T. (
1997
). Modulation of embryonic intracellular Ca2+signaling by Wnt-5A.
Dev. Biol.
182
,
114
-120.
Umesono, Y., Watanabe, K. and Agata. K.(
1999
).Distinct structural domains in the planarian brain defined by the expression of evolutionarily conserved homeobox genes.
Dev. Genes Evol.
209
,
31
-39.
Wallingford, J. B., Vogeli, K. M. and Harland, R. M.(
2001
). Regulation of convergent extension in Xenopus by Wnt5a and Frizzled-8 is independent of the canonical Wnt pathway.
Int. J. Dev. Biol.
45
,
225
-227.
Witze, E. S., Litman, E. S., Argast, G. M., Moon, R. T. and Ahn,N. G. (
2008
). Wnt5a control of cell polarity and directional movement by polarized redistribution of adhesion receptors.
Science
320
,
365
-369.
Wong, G. T., Gavin, B. J. and McMahon, A. P.(
1994
). Differential transformation of mammary epithelial cells by Wnt genes.
Mol. Cell. Biol.
14
,
6278
-6286.
Yoshikawa, S., McKinnon, R. D., Kokel, M. and Thomas, J. B.(
2003
). Wnt-mediated axon guidance via the Drosophila Derailed receptor.
Nature
422
,
583
-588.
Zhang, X., Zhu, J., Yang, G. Y., Wang, Q. J., Qian, L., Chen, Y. M., Chen, F., Tao, Y., Hu, H. S., Wang, T. and Luo, Z.(
2007
). Dishevelled promotes axon differentiation by regulating atypical protein kinase C.
Nat. Cell Biol.
9
,
743
-754.
© 2009.
2009

Supplementary information

Supplemental Figure S1

Fig. S1. Sequence analysis of the Smed-Evi protein. (A) Alignment of Evi proteins from different species, showing four conserved cysteines (pink), and eight putative transmembrane domains (blue asterisks). Smed-Evi transmembrane domains were predicted with the help of TMpred (http://www.ch.embnet.org/software/TMPRED_form.html). (B) Phylogenetic tree of Evi proteins inferred from the accurate multiple amino-acid sequence of Evi proteins obtained using the MAFFT version 5.8 (http://align.bmr.kyushu-u.ac.jp/mafft/online/server/). The CAT+Γ model in an MCMC framework, as implemented in PhyloBayes (http://www.lirmm.fr/mab/). The complete Evi/Wls amino acid sequences were used. Smed-Evi groups with invertebrate members. Its closer position to Ce-Evi/Wls is probably due to the phenomenon of �long branch attraction�. No Evi protein from any other Lophotrocozoan has been reported. Ag, Aedes aegypti; Ce, Caenorhabditis elegans; Ci, Ciona intestinalis; Dm, Drosophila melanogaster; Dr, Danio rerio; Hs, Homo sapiens; Mm, Mus musculus; Sp, Strongylocentrotus purpuratus; Tc, Tribolium castaneum; Xl, Xenopus laevis. Accession numbers: Ag-Evi/Wls, XP_001237950; Ce-Evi/Wls, NP_001022275; Ci-Evi/Wls, XP_002123798; Dm-Evi/Wls, NP_729681; Dr-Evi/Wls, NP_998311; Hs-Evi/Wls, NP_079187; Mm-Evi/Wls, NP_080858; Sp-Evi/Wls, XP_001181848; Tc-Evi/Wls, XP_974084; Xl-Evi/Wls, Q66IZ4.

- pdf file
Supplemental Figure S2

Fig. S2. Phenotypic scoring of regenerating Smed-evi RNAi animals. Alive regenerating heads, trunks and tail fragments of Smed-evi RNAi animals where analyzed with a stereomicroscope. (A,A′) All regenerated head fragments showed differentiation of two or more ectopic posterior eyes and two lateral protrusions in the middle region of the animal (A′). (B-H) Bipolar regenerated trunks showed different phenotypes, depending on RNAi penetrance but also on frequent spontaneous scission during regeneration. At early stages of regeneration, all trunk fragments showed ectopic anterior eyes. However, the severity of the phenotype on the posterior part of the animal was different, giving rise to: �tailless� phenotype, without ectopic posterior eyes (C); �two-headed� phenotype with several ectopic anterior eyes, and two posterior ectopic eyes (D); and �two-headed� phenotype with several ectopic anterior and posterior eyes (E). Approximately 50% of the �two-headed� animals underwent spontaneous scission, giving rise to an anterior part, which generated another �tailless� phenotype (F), or even a secondary posterior head (G). The posterior fragment generated after scission was not able to regenerate a normal anterior head, and remained single-headed, with multiple posterior eyes (H). In all cases, animals had two lateral protrusions in the middle region of the body, which never showed ectopic eyes. (I,I′) Each regenerated tail fragment had ectopic anterior eyes, and a �heart-like� shape, due to a tissue regression of the tail region (I′). (J) Quantification of phenotypes. Planarians with an ectopic posterior head, in which two eyes were detected, are named �Two- headed�. When additional anterior or posterior eyes appeared, we refer to the phenotype as �Two-headed with ectopic anterior/posterior eyes�. Red arrows indicate ectopic eyes. Yellow arrows indicate normal anterior eyes. Orange arrowheads point at lateral protrusions. Scale bar: 300 µm in A-B′; 500 µm in C-I.

- pdf file
Supplemental Figure S3

Fig. S3. The dorsoventral axial patterning is not affected in Smed-evi-silenced planarians. (A-D) Whole-mount in situ hybridization analysis of dorsal (septin) and ventral (eye53) marker mRNAs in bipolar regenerating trunk fragments on day 20 after amputation. (A,B) Dorsal and ventral views of control animals; (C,D) Smed-evi-silenced animals. Note, that the distribution of neither marker is changed in the absence of Smed-evi. Scale bar: 500 µm.

- pdf file
Supplemental Figure S5

Fig. S5. Expression analysis and functional characterization of Smed-wntA. (A,A′) Smed-wntA mRNA expression in intact animals. Smed-wntA is expressed in the posterior region of the cephalic ganglia (yellow arrowheads in A,A′), in the ventral nerve cords (white arrows) and in the pharynx (white asterisk). (B) Smed-wntA mRNA expression during regeneration. In head fragments, which must regenerate the rest of the body, Smed-wntA is detected in the posterior region of the cephalic ganglia (yellow arrowheads) and in the primordial of the pharynx (orange arrowhead). In bipolar regenerating fragments, Smed-wntA mRNA is detected in the new nervous tissue, both in the anterior (yellow arrows) and in the posterior blastema (white arrows), and also in the pharynx (white asterisk) and the mouth (red arrowhead). Its expression is not detected in tail fragments, which must regenerate the rest of the body, at 4 days after dissection. (C-E) Phenotype of Smed-wntA-silenced planarians. After 20 days of regeneration, Smed-wntA-silenced planarians show a defect in the shape of the new head, as it seems smaller and more round (C). Analysis with molecular markers shows that the brain of Smed-wntA-silenced animals is expanded posteriorly (gluR and DAPI), and that brain branches have an irregular shape (gluR; D,E). Immunodetection of Arrestin (VC-1) shows that the visual axons are also expanded posteriorly (red arrowheads; E). Even though the posterior expansion of the brain is similar to that of evi RNAi animals, the elongated visual axons after wntA knockdown are not evident in evi RNAi animals, probably because of the complexity of the phenotype. Scale bar: 500 µm in A; 300 µm in B; 250 µm in A′,C. Our results agree with the phenotype reported after DjwntA RNAi (Kobayashi et al., 2007). DjwntA-silenced planarians also show an expansion of the brain, with differentiation of ectopic and irregular brain branches. However, in the reported study, the analysis with different molecular markers suggests that the expanded region corresponds to the anterior part of the ganglia, resulting in the expansion of the visual center and the appearance of several ectopic eyes. We did not observe differentiation of ectopic eyes in S. mediterranea. More molecular markers should be used in order to address this issue.

- pdf file
Supplemental Table S1- pdf file
Supplemental Figure S4

Fig. S4. Phylogenetic analysis of the S. mediterranea Wnt family. Phylogenetic tree inferred from the accurate multiple amino-acid sequence alignment of Wnt proteins using MAFFT version 5.8 (http://align.bmr.kyushu-u.ac.jp/mafft/online/server/). The CAT+Γ model in an MCMC framework, as implemented in PhyloBayes (http://www.lirmm.fr/mab/) was used. Only the Wnt domain, as determined in SMART (http://smart.embl-heidelberg.de) and the Protein families database (http://www.sanger.ac.uk/Software/Pfam/index.shtml), was used. Confidence values are indicated in the main nodes. Smed-Wnt5 is the only S. mediterranea Wnt that clusters with one of the already described Wnt subfamily (Wnt5) with a high confidence value. Smed-Wnt2-1, together with Dj-WntB (the homolog from the planarian species Dugesia japonica) and Sj-Wnt10 (from Schistosoma japonicum, also a Platyhelminth) cluster into the Wnt2 subfamily; Smed-Wnt11-1 and Smed-Wnt11-2 into the Wnt11 subfamily. Although with a low confidence value, both results are reproducible when inferring different phylogenetic trees. Smed-WntA, Smed-WntP-2 and Smed-WntP-3 cluster with Dj-WntA and Sj-Wnt4 (from Dugesia japonica and Schistosoma japonicum, Platyhelminthes), but do not group with any of the already described Wnt subfamilies. Smed-WntP-1 and Smed-WntP-4 cluster, but also do not fall into any of the already described Wnt subfamilies. The clustering of Nv-WntA with Smed-WntP-1 and Smed-WntP-4 is probably due to the phenomenon of �long branch attraction�. S. mediterranea Wnts are labeled with a red circle. Ag, Anopheles Gambia; Bf, Branchiostoma floridae; Ce, Caenorhabditis elegans; Dj, Dugesia japonica; Gt, Girardia tigrina; Hs, Homo sapiens; Nv, Nematostella vectensis; Pd, Platynereis dumerilii; Pv, Patella vulgata; Sj, Schistosoma japonicum; Smed, Schmidtea mediterranea; Sp, Strongylocentrotus purpuratus; Tc, Tribolium castaneum. Accession numbers: Ag-Wnt1, XP_553580; Ag-Wnt10, XP_318815; Ag-Wnt5, XP_319487; Ag-Wnt6, XP_318816; Ag-Wnt7, XP_001238162; Ag-Wnt9, XP_318818; Ag-WntA, XP_557821; Bf-Wnt1, AAC80432; Bf-Wnt11, AAF80555; Bf-Wnt3, AAL37555; Bf-Wnt4, AAC80431; Bf-Wnt5, AAL37556; Bf-Wnt7b, AAC80433; Bf-Wnt8, AAF80559; Ce-cWn-1, NP_493668; Ce-cWn-2, NP_501822; Ce-egl-20, NP_501754; Ce-lin-44, NP_001021081; Ce-mom-2, NP_505154; Dj-WntA, BAD93239; Dj-WNTB, BAD93245; Gt-Wnt5, AAO17782; Hs-Wnt1, NP_005421; Hs-Wnt10a, NP_079492; Hs-Wnt11, CAA73223; Hs-Wnt16, NP_476509; Hs-Wnt2b, NP_004176; Hs-Wnt3a, AAI03922; Hs-Wnt4, NP_110388; Hs-Wnt5A, NP_003383; Hs-Wnt6, NP_006513; Hs-Wnt7b, NP_478679; Hs-Wnt8a, Q9H1J5; Hs-Wnt9A, NP_003386; Hs-Wnt9B, O14905; Nv-Wnt1, AAT00640; Nv-Wnt10, AAT00641; Nv-Wnt11, AAV87175; Nv-Wnt16, ABF48091; Nv-Wnt2, AAW28132;Nv-Wnt3, ABF48092; Nv-Wnt4, AAV87174; Nv-Wnt6, AAW28134; Nv-Wnt7, AAV87176; Nv-Wnt8, AAW28136; Nv-WntA, AAT02182; Pd-Wnt1, CAD37164; Pd-Wnt4, CAD37166; Pd-WntA, CAD37169; Pv-Wnt1, CAD37170; Pv-Wnt10, CAD37172; Pv-Wnt2, CAD37171; Pv-WntA, CAD37173; Sj-Wnt10, ABG73039; Sj-Wnt4, ABG73038; Smed-Wnt2-1, FJ463753; Smed-Wnt11-1, ABY85210; Smed-WntP-1, ABY85207; Smed-WntP-2, ABY85208; Smed-WntP-3, ABY85209; Sp-Wnt1, NP_001116972; Sp-Wnt10, XP_781564; Sp-Wnt3, XP_790595; Sp-Wnt4, XP_797603; Sp-Wnt4b, XP_786346; Sp-Wnt5, XP_779946; Sp-Wnt6, XP_790077; Sp-Wnt7, XP_796616; Sp-Wnt7b, XP_787051; Sp-Wnt8, NP_999832; Tc-Wnt1, NP_001107822; Tc-Wnt10, XP_968210; Tc-Wnt11, XP_969261; Tc-Wnt5, XP_974684; Tc-Wnt6, XP_968055; Tc-Wnt7, XP_973159; Tc-Wnt9, XP_967898; Tc-WntA, XP_972893; Tc-WntD/8, XP_971439.

- pdf file
Movie 1

Movie 1. Confocal sections through the brain of a wild-type regenerating head fragment. Confocal sections correspond to the head region of a head fragment, which must regenerate the rest of the body, of a control animal that was immunostained with an anti-Synapsin antibody. From dorsal to ventral. Magnification: 40×.

- avi file
Movie 2

Movie 2. Confocal sections through the ectopic posterior brain of a regenerating Smed-evi RNAi head fragment. Confocal sections correspond to the regenerating region of a head fragment, immunostained with an anti-Synapsin antibody. From dorsal to ventral. Magnification: 40×.

- avi file
Movie 3

Movie 3. Confocal sections through the brain of a wild-type regenerating trunk fragment. Confocal sections correspond to the head region of a bipolar regenerating control animal immunostained with an anti-Synapsin antibody. From ventral to dorsal. Magnification: 20×.

- avi file
Movie 4

Movie 4. Confocal sections through the anterior brain of a regenerating Smed-evi RNAi trunk fragment. Confocal sections correspond to the anterior region of a bipolar regenerating Smed-evi RNAi animal immunostained with an anti-Synapsin antibody. From ventral to dorsal. Magnification: 20×.

- avi file
Movie 5

Movie 5. Confocal sections through the brain of a regenerating Smed-wnt5 RNAi trunk fragment. Confocal sections correspond to the head region of a bipolar regenerating Smed-wnt5 RNAi animal immunostained with an anti-Synapsin antibody. From ventral to dorsal. Magnification: 20×.

- avi file