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The Journal of Neuroscience, July 2, 2003, 23(13):5507-5519
Previous Article | Next Article
Genetic Analysis of the Roles of Hh, FGF8, and Nodal Signaling during Catecholaminergic System Development in the Zebrafish Brain
Jochen Holzschuh, Giselbert Hauptmann, andWolfgang Driever Developmental Biology, Institute Biology 1, University of Freiburg, D-79104 Freiburg, Germany
Abstract
Top
Abstract
Introduction
CNS catecholaminergic neurons can be distinguished by their neurotransmitters as dopaminergic or noradrenergic and form in distinct regions at characteristic embryonic stages. This raises the question of whether all catecholaminergic neurons of one transmitter type are specified by the same set of factors. Therefore, we performed genetic analyses to define signaling requirements for the specification of distinct clusters of catecholaminergic neurons in zebrafish. In mutants affecting midbrain– hindbrain boundary (MHB) organizer formation, the earliest ventral diencephalic dopaminergic neurons appear normal. However, after 2 d of development, we observed fewer cells than in wild types, which suggests that the MHB provides proliferation or survival factors rather than specifying ventral diencephalic dopaminergic clusters. In hedgehog (Hh) pathway mutants, the formation of catecholaminergic neurons is affected only in the pretectal cluster. Surprisingly, neither fibroblast growth factor 8 (FGF8) alone nor in combination with Hh signaling is required for specification of early developing dopaminergic neurons. We analyzed the formation of prosomeric territories in the forebrain of Hh and Nodal pathway mutants to determine whether the absence of specific dopaminergic clusters may be caused by early patterning defects ablating corresponding parts of the CNS. In Nodal pathway mutants, ventral diencephalic and pretectal catecholaminergic neurons fail to develop, whereas both anatomical structures form at least in part. This suggests that Nodal signaling is required for catecholaminergic neuron specification. In summary, our results do not support the previously suggested dominant roles for sonic hedgehog and Fgf8 in specification of the first catecholaminergic neurons, but instead indicate a novel role for Nodal signaling in this process.
Key words: catecholaminergic system; dopaminergic neurons; Danio rerio; sonic hedgehog; nodal; fibroblast growth factor 8; forebrain; pretectum; hypothalamus; locus coeruleus; medulla oblongata
Introduction
The vertebrate CNS catecholaminergic (CA) system participates in a variety of tasks including motor coordination, mood regulation, and cognitive function. Reflecting the complexity of the CA system, distinct groups of CA neurons form at various developmental stages (for review, see Smeets and Reiner, 1994). Several transcription factors have been shown to contribute to their specification, including Ptx3 (Smidt et al., 1997
Zebrafish is a model organism well suited for genetic analysis of CA system development, with a large number of available mutations affecting signaling pathways and the opportunity to perform forward genetic screens. During a mutagenesis screen, several mutants with abnormal tyrosine hydroxylase expression (TH; the rate-limiting enzyme in catecholamine biosynthesis) were isolated (Guo et al., 1999a
Here, we investigate the influence of mutations affecting signaling pathways or centers that have been implicated previously in vertebrate CA development. We study the influence of mutations affecting Hh and FGF8 signaling as well as those affecting MHB development. Because Activin has been suggested to regulate TH expression in basal forebrain progenitors (Daadi et al., 1998
(TGF
Materials and Methods
Zebrafish maintenance and strains. Zebrafish were maintained under standard laboratory conditions at 28.5°C (Westerfield, 1995In zebrafish, by the end of gastrulation, oep, cyc, squint (sqt; nodal-related factor), and sur are expressed in the prechordal and posterior mesendoderm and later become restricted to the epiphysal region of the dorsal diencephalon during somitogenesis (Rebagliati et al., 1998
Anatomical nomenclature. Zebrafish central CA neuronal clusters are named according to Guo et al. (1999a
Whole-mount in situ hybridization. Standard methods for whole-mount in situ hybridization were used (Hauptmann and Gerster, 1994
Results
The first dopaminergic neurons in zebrafish differentiate along the alar–basal boundary of the posterior tuberculum
To better understand the specific signaling environment in which the various CA neuronal groups develop, we determined where these neurons differentiate relative to developmental boundaries and signaling centers. In the early embryonic zebrafish brain, few morphological landmarks exist to determine the exact location of neuronal groups. Thus, we used the expression domains of regulatory genes known to subdivide the embryonic forebrain as topological markers (Macdonald et al., 1994
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Figure 1. The first dopaminergic neurons differentiate in the diencephalic posterior tuberculum. Visualization of forebrain gene expression domains and th expression by double in situ hybridization of whole-mount wild-type embryos are shown. A–E, Lateral views of the brain (anterior is to the left, dorsal is to the top). In situ hybridization of 24 hpf embryos with dbx1a (A), dlx2 (B), foxa1 (C), pax6.1 (D), and shh (E) is shown in red, and th is in blue. For better visibility, the skin, eyes, and yolk have been removed except in C where only the yolk has been removed. A, The ventral part of the most anterior transverse dbx1a expression domain marks the caudal hypothalamus. B, The DA neurons are located within the dlx2 expression domain in the hypothalamus. C, The DA cluster extends caudally to the anterior end of the longitudinal expression domain of foxa2 (arrowhead indicates the midbrain– hindbrain boundary). D, The DA cluster extends longitudinally close to the ventral edge of the alar plate (ventral border of pax 6.1 expression) in the basal plate marked by the shh expression domain (E). dt, Dorsal thalamus; hy, hypothalamus; pr, pretectum; pt, posterior tuberculum; t, telencephalon; vt, ventral thalamus; zl, zona limitans intrathalamica.
FGF8 signaling is not required for differentiation of the first dopaminergic neurons
Previous studies showed that FGF8-soaked beads can induce differentiation of DA neurons in explant cultures from embryonic rat brain, whereas DA differentiation can be prevented by introducing dominant-negative FGF receptors (Ye et al., 1998
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Figure 2. Formation of dopaminergic groups is not affected in ace/fgf8 mutant embryos. A–H, Whole-mount in situ hybridization for th expression in wild-type (A, C, E, G) and ace mutant embryos (B, D, F, H). A–H, Dorsal views; anterior is to the left. A, B, The first th-expressing dopaminergic neurons appear normal in ace mutants at 24 hpf. C, D, At 72 hpf, fewer dopaminergic neurons are seen in the ventral diencephalon of ace mutants compared with that of wild-type embryos, whereas th expression appears normal in the pretectum and olfactory bulbs (E–H). E, F, The noradrenergic neurons of the LC are absent in ace mutants. vDD, Ventral diencephalic dopaminergic neurons; ObC, olfactory bulb catecholaminergic neurons; PrC, pretectal catecholaminergic neurons. Scale bars, 50 µm.
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Table 1. Effects of hedgehog, FGF8, and Nodal pathway mutants on the formation of the main dopaminergic and noradrenergic groups in the zebrafish CNS
The only other characterized member of the FGF8/17/18 subgroup of Fgfs in zebrafish is an ortholog to mammalian Fgf17. Zebrafish fgf17 is coexpressed with fgf8 in the MHB from approximately the 8-somite stage onwards (Reifers et al., 2000
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Figure 3. The LC is absent and the ventral diencephalic dopaminergic neurons are slightly reduced in noi/pax2.1 mutant embryos. Whole-mount in situ hybridization for dat in wild-type (A, B, E, F) and noi/pax2.1 (C, D, G, H) mutant embryos. A, C, Lateral views, dorsal is to the top. B, D, E–H, Dorsal views, anterior is to the left. A–D, At 48 hpf, the dat expression pattern reveals a slight decrease in ventral diencephalic dopaminergic neurons in noi mutant embryos. E–H, The catecholaminergic neurons in the olfactory bulb and pretectum appear normal in noi mutant embryos. F, H, In noi mutant embryos, the LC is absent. vDD, Ventral diencephalic dopaminergic neurons; ObD, olfactory bulb catecholaminergic neurons; PrC, pretectal catecholaminergic neurons. Scale bars, 30 µm.
To reveal possible redundant functions of FGF8 and FGF17, we analyzed th and dat expression in ace noi double mutant embryos that lack expression of both FGF8 and FGF17 (data not shown). Among 100 progeny from an intercross of ace noi double heterozygous fish, we found none with a CA phenotype more severe than that of ace or noi single mutant embryos; all progeny developed DAT-expressing cells in the ventral diencephalon, pretectum, and olfactory bulb. Thus, our results indicate that FGF8 and FGF17 are not strictly required for DA neuron formation in the forebrain and do not act redundantly in this process. In contrast, our results confirm a requirement for FGF8 during CA neuron development in the locus coeruleus.
Although both noi and ace mutants fail to maintain the MHB organizer, these mutations do not affect its initial establishment. To elucidate potential early roles of the MHB in CA system development, we analyzed spiel ohne grenzen mutant embryos, which fail to establish the MHB. spg is required early during MHB establishment and encodes the zebrafish pou2 gene (Belting et al., 2001
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Figure 4. The catecholaminergic neurons in the diencephalon are reduced and the LC is absent in spg mutant embryos. A–F, th expression in the forebrain and hindbrain of wild-type (A, C, D) and spg (B, E, F) mutant embryos at 3 dpf. A–F, Dorsal views, anterior is to the left. In spg mutant embryos (B), the catecholaminergic neurons of the LC are absent and those of the diencephalon are reduced, whereas the remaining hindbrain CA clusters develop normally (E, F). AP, Area postrema; vDD, ventral diencephalic dopaminergic neurons; MC, medullary catecholaminergic neurons; ObC, olfactory bulb catecholaminergic neurons; white arrows indicate the absence of the LC.
POU domain proteins have been implicated in catecholaminergic and serotonergic neuronal differentiation in invertebrates (Johnson and Hirsh, 1990
Shh is required for DA neuron development in the diencephalic alar plate but not in the basal plate
We investigated whether lack of Shh signaling can affect DA neuron differentiation in zebrafish mutants. The zebrafish syu locus encodes the ortholog of the mammalian Shh gene (Schauerte et al., 1998
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Figure 5. The pretectal catecholaminergic neurons and the amacrine cells of the retina are affected in hedgehog pathway mutants. A–F, th expression at 3 dpf in wild-type (A, B) and syu (C–F) mutant embryos (lateral views, anterior is to the left, dorsal is to the top). A, C, E, The pretectal cluster of catecholaminergic neurons is reduced (C) or absent (E, white arrow) in syu mutant embryos. The dopaminergic cell cluster in the ventral diencephalon is altered in morphology but not in size in syu mutant embryos. D, F, Dopaminergic amacrine cells are reduced (D) or absent (F, white arrowhead) in syu mutant embryos. G–J, dopamine transporter expression in 3 dpf embryos. G–J, Lateral views (G,I) and dorsal views (H, J); anterior is to the left. G, I, Of the CNS dopaminergic clusters, only the pretectal cluster is affected in smu mutants. H, J, The dopaminergic amacrine cells are reduced and the dat-expressing reticular astrocytes are absent in smu mutant embryos (J, white arrows). AD, Amacrine dopaminergic neurons; vDD, ventral diencephalic dopaminergic neurons; ObC, olfactory bulb catecholaminergic neurons; PrC, pretectal catecholaminergic neurons.
Two additional hedgehog genes exist in zebrafish, tiggy-winkle hedgehog (tww) (Ekker et al., 1995
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Figure 6. smu/smoh and ace/fgf8 double mutants develop additive DA neuronal phenotypes. A, C, E, G, dat expression or th expression (B, D, F, H). A–H, Lateral views, anterior to the left, dorsal is to the top. In smu/smoh (C), ace/fgf8 (E), and smu ace (G) double mutants, the earliest developing dopaminergic neurons in the ventral diencephalon appear normal when compared with wild-type embryos (A). By 48 hpf, additive phenotypes are observed in smu ace double mutants (H); the ventral diencephalic cluster is misshapen as in smu mutants (D) and the LC is absent as in ace (F). Insets in B, D, F, and H show higher magnification views of the region of the locus coeruleus. vDD, Ventral diencephalic dopaminergic neurons. White arrows indicate the absence of the LC.
In the retinae of both syu and smu mutants, dat-expressing amacrine cells are absent or reduced in number, indicating a defect in DA amacrine cell differentiation (Fig. 5D,F,H,J). The absence of dat-expressing reticular astrocytes surrounding the optic nerve in these mutants indicates that the development of these cells also depends on Hh signaling (Fig. 5H,J).
shh and fgf8 double mutants do not reveal synergistic effects in DA system development
Our analysis of syu/shh, smu/smoh, and ace/fgf8 mutant embryos reveals that DA neurons successfully develop in the diencephalon in the absence of either Shh or FGF8 signaling. To examine whether these two signaling pathways interact to specify DA neurons, we generated double mutants for smu and ace and examined the expression of th and dat. The expression of dat in the ventral diencephalon of smu ace double mutants at 24 hpf is similar to that in wild-type embryos (Fig. 6A,G). By 2 dpf, we detected changes in th expression in smu ace double mutants, which are additive with respect to the single mutant phenotypes of smu or ace (Fig. 6B,D,F,H). The smu ace double mutants lack the locus coeruleus, as do ace mutants, and show an altered morphology in the ventral diencephalic DA cluster, as do smu mutants. By 3 dpf, the smu ace double mutants have begun to degenerate, preventing additional investigation of DA system development. Together, our data indicate that the earliest differentiation of ventral diencephalic DA neurons (20–40 hpf) does not depend on either Hh or Fgf8 signaling alone, or in combination.Differentiation of CA neurons of the basal and alar plate is affected in Nodal pathway mutants
A subset of dopaminergic neurons in C. elegans depends on a functional TGFcyc encodes the Nodal-related protein Ndr2 (Rebagliati et al., 1998
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Figure 7. Nodal pathway mutants affect the development of the ventral diencephalic and pretectal catecholaminergic neurons. A–E, th expression revealing the effects of mutations within the Nodal pathway on catecholaminergic neuron development (lateral views, anterior is to the left). A, D, th expression in wild-type embryos at 72 and 48 hpf, respectively. B, In cyc mutant embryos, both the ventral diencephalic DA neurons and the catecholaminergic neurons of the pretectum fail to develop, whereas the CA neurons in the hindbrain are unaffected. C, By 72 hpf, oep mutants lack diencephalic catecholaminergic neurons, whereas those of the hindbrain clusters are formed. E, By 48 hpf, MZsur mutant embryos develop few-to-no catecholaminergic neurons in the diencephalon, whereas the LC appears normal. White arrows indicate absence of PrC; white arrowheads indicate absence of vDD. AD, Amacrine dopaminergic neurons; vDD, ventral diencephalic dopaminergic neurons; MC, medulla oblongata catecholaminergic neurons; PrC, pretectal catecholaminergic neurons. Scale bars, 100 µm.
The zebrafish membrane-bound EGF-CFC (epidermal growth factor–Cripto, Frl-1, and Cryptic family member) protein Oep is required for the reception of Nodal signals (Zhang et al., 1998
The zebrafish transcription factor Sur/FoxH1/Fast1 is a nuclear signal transducer for Nodal signaling (Pogoda et al., 2000
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Figure 8. Formation of catecholaminergic neurons is affected in the ventral diencephalon of Zsur mutant embryos. A–J, Lateral views (A–F) (anterior is to the left, dorsal is to the top) and dorsal views (G–J) of th expression in the brain of wild-type (A, C, E, G,I) and Zsur mutant (B, D, F, H,J) embryos at 3 dpf. A–F, Overview of the catecholaminergic neurons (A, B), olfactory bulbs (C,D), and pretectum (E, F). In the ventral diencephalon of Zsur mutant embryos, the dopaminergic neurons are reduced in the posterior tuberculum (G,H) and hypothalamus (I, J). The LC (G, H) develops normally in Zsur mutants. vDD, Ventral diencephalic dopaminergic neurons; ObC, olfactory bulb catecholaminergic neurons; PrC, pretectal catecholaminergic neurons. Scale bars, 17 µm.
Together, these findings indicate that the Nodal pathway is not only required for the early establishment of the hypothalamus (Varga et al., 1999
Nodal and Hh pathway mutants affect early patterning of the ventral forebrain but not the pretectum
The pretectal and hypothalamic CA system defects in Hh and Nodal signaling pathway mutants could be caused either indirectly by early patterning defects that prevent development of the respective brain regions, or by a more direct involvement of Hh and Nodal signaling in CA neuron specification. To distinguish between these possibilities, we investigated forebrain patterning in these mutants by visualizing region-specific expression domains of hlx1/dbx1a, dlx2, and shh at 24 hpf, the time of CA neuron formation.In MZ sur mutants, dlx2 and shh are expressed in the diencephalon, but the most anterior domains of expression are lost. The remaining domains enclose the posterior tuberculum in which DA neurons differentiate (Fig. 9D,E). The hlx1/dbx1a domains in the posterior tuberculum and the pretectum are unchanged (Fig. 9C,F). In contrast, in the more severe Nodal pathway mutants oep and cyc, the hypothalamic expression domains of hlx1/dbx1a, dlx2, and shh do not form (Fig. 9G–L), whereas hlx1/dbx1a expression does occur in the pretectum (Fig. 9I,L).
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Figure 9. Embryonic patterning defects in the diencephalon of Nodal pathway and smu mutants. A–O, Embryos at 24 hpf (lateral views; anterior is to the left, dorsal is to the top). A–C, Wild-type embryos showing the expression domains of shh (A), dlx2 (B), and dbx1a (C). D–F, In MZsur embryos, shh expression is maintained in the zona limitans, part of the hypothalamus and midline (D), the expression domain of dlx2 in the hypothalamus is reduced in size (E); and the dbx1a expression domains in the pretectum and ventral diencephalon are present (F). G–I, oep mutant embryos show no hypothalamic expression of shh (G), dlx2 (H), and dbx1a (I), whereas the pretectal dbx1a domain is present. J–L, In cyc mutant embryos, expression of shh (J), the ventral expression domains of dlx2 (K), and dbx1a (L) in the forebrain are absent, whereas dbx1a expression in the pretectum is present. M–O, In smu mutant embryos, the expression of shh (M) in the zona limitans is absent, but a reduced expression in the ventral brain remains. The hypothalamic expression domains of dlx2 (N) and dbx1a (O), as well as the pretectal dbx1a domain can still be detected. The black arrows indicate the expression domain of shh in the ventral diencephalons. White arrowheads point to the dlx2 domain and white arrows point to the dbx1a domain in the ventral diencephalons. The red stars indicate the expression domain of dbx1a in the pretectum.
smu mutants show no shh expression in the zona limitans with reduced expression in the midline (Fig. 9M). The expression domain of dlx2 that marks the anterior boundary of prosomere 3 is present in smu mutants (Fig. 9N) (Varga et al., 2001
The expression domains of hlx1/dbx1a are expanded ventrally into the basal plate in both Nodal pathway and smu mutant embryos (Fig. 9C,F,I,L,O), consistent with the dorsal–ventral patterning defects in those mutants. Interestingly, in Mzsur, oep, and cyc mutants, the hlx1/dbx1a domain is also expanded in the dorsal midbrain. A summary of the early neural patterning defects correlated with the neuronal phenotype in Nodal pathway mutants is provided in Table 2.
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Table 2. Comparison of CA neuronal cluster development and early neural patterning defects in the diencephalon of Nodal pathway and smu mutant embryos
Our analysis of pattern formation in the CNS of mutant embryos indicates that the pretectum develops normally in Nodal and Hh pathway mutants. We can then exclude the possibility that the defects in CA neuron specification in the pretectum are caused indirectly by early patterning defects and subsequent loss of the pretectum. In addition, the expression domains of shh, dlx2, and hlx1/dbx1a observed in the hypothalamic region of Mzsur mutant embryos indicate that the diencephalic territories in which DA neurons normally would form are present in the mutant embryos. Thus, Nodal signaling may also be directly involved in DA neuron differentiation in the ventral diencephalon.
Discussion
It has been hypothesized that, in mammals, all DA neuron progenitors arise from two regions, the telencephalic and diencephalic area near the anterior neural ridge (ANR) and the midbrain, rostral to the MHB and that all of these progenitors depend on Shh signaling from the midline and Fgf8 signaling from the MHB and ANR (Hynes and Rosenthal, 1999FGF8 and the MHB are not strictly required for DA neuron differentiation in zebrafish
A role of FGF8 and Shh in regulating DA cell specification was postulated, primarily on the basis of experiments using cell and explant cultures of chicken, mouse, and rat brains (Hynes et al., 1995aBoth in vivo and in vitro analyses of mammalian brain development also support the conclusion that Fgf8 and Shh are not required for DA neuronal fate specification. The MHB, the source of FGF8 suggested to be important for midbrain DA neuronal development, is absent in engrailed-1 mutant mice (Wurst et al., 1994
DA specification in the pretectum and ventral diencephalon requires Nodal signaling
We observed little to no DA–NA neurons in the pretectal area and ventral diencephalon in zebrafish nodal pathway mutants lacking the Cyc/Ndr2 signal, Nodal coreceptor Oep, or downstream transcription factor Sur/FoxH1. In cyc and oep mutant embryos, the ventral diencephalon, including the hypothalamus and basal plate portion of p3, fails to form (Varga et al., 1999Cell and tissue culture studies have shown that ligands of the TGF
Alternatively, because the nodal-related genes cyc and sqt, as well as the receptor oep and signal transducer sur, are not expressed at late stages in the ventral diencephalon, the Nodal/TGF
Formation of pretectal CA neurons depends on Hh and Nodal signaling
Formation of the pretectal DA–NA neurons requires Hh and Nodal signaling. In mutants affecting either signaling pathway, the pretectal cluster of DA–NA neurons is reduced or deleted. Hh signaling has been shown to act downstream of Nodal signaling in patterning the telencephalon (Rohr et al., 2001In summary, our comprehensive lack-of-function in vivo genetic data provide the novel opportunity to evaluate the contributions of various signaling pathways and signaling centers to the development of the CA system. Our findings indicate that the previously dominating concept in which an epigenetic grid of Shh and FGF8 specified all DA neurons is unlikely, and suggest a new signaling framework in which a prepattern evolved in the neurectoderm during gastrulation, followed by Nodal, Shh, FGF8, and other signals, specifies the earliest DA and NA neurons in the forebrain and anterior hindbrain.
Footnotes
Received Nov. 7, 2002; revised Apr. 10, 2003; accepted Apr. 14, 2003.This work was supported by Deutsche Forschungsgemeinschaft Grants SFB 505 TP B7 and SFB 592 TP A3 (W.D.). We thank Dr. Z. Varga for complementation with smub641, Dr. D. Meyer for MZsur fish, and A. Fiebig for help during the initial phase of the project. We thank Dr. S. Ryu, Dr. Z. Varga, Dr. K. Lunde, Dr. D. Meyer, and K. Dürr for helpful critique of this manuscript and discussion. S. Götter and R. Schlenvogt provided expert care of the fish.
Correspondence should be addressed to Dr. W. Driever, Developmental Biology, Institute Biology 1, University of Freiburg, Hauptstrasse 1, D-79104 Freiburg, Germany. E-mail: driever{at}biologie.uni-freiburg.de.
J. Holzschuh's present address: Department of Developmental and Cell Biology, University of California, Irvine, CA 92697.
Copyright © 2003 Society for Neuroscience 0270-6474/03/235507-13$15.00/0
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