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The Journal of Neuroscience, September 1, 2000, 20(17):6501-6516
Defects of Tyrosine Hydroxylase-Immunoreactive Neurons in the Brains of Mice Lacking the Transcription Factor Pax6
Tania Vitalis1, Olivier Cases1, 2, Dieter Engelkamp3, Catherine Verney2, and David J. Price1 1 Department of Biomedical Sciences, Medical School, Edinburgh EH8 9AG, Scotland, 2 Institut National de la Santé et de la Recherche Médicale U106, Hôpital de la Salpêtrière, 75651 Paris Cedex 13, France, and 3 Medical Research Council Human Genetics Unit, Western General Hospital, Edinburgh, EH4 2XU, Scotland
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
In the CNS, the lack of the transcription factor Pax6 has been associated with early defects in cell proliferation, cell specification, and axonal pathfinding of discrete neuronal populations. In this study, we show that Pax6 is expressed in discrete catecholaminergic neuronal populations of the developing ventral thalamus, hypothalamus, and telencephalon. In mice lacking Pax6, these catecholaminergic populations develop abnormally: those in the telencephalon are reduced in cell number or absent, whereas those in the ventral thalamus and hypothalamus are greatly displaced and densely packed. Catecholaminergic neurons of the substantia nigra (SN) and the ventral tegmental area (VTA) do not express Pax6 protein. Nevertheless, mice lacking Pax6 display an altered pathfinding of SN-VTA projections: instead of following the route of the medial forebrain bundle ventrally, most of the SN-VTA projections are deflected dorsorostrally at the pretectal-dorsal thalamic transition zone and in the dorsal thalamic alar plate. Moreover, some catecholaminergic neurons are displaced dorsally to an ectopic location at the pretectal-dorsal thalamic transition zone. Interestingly, from the pretectal-dorsal thalamic to the dorsal thalamic-ventral thalamic transition zones, mice lacking Pax6 display an ectopic ventral to dorsal expansion of the chemorepellant/chemoattractive molecule, Netrin-1. This may be responsible for both the altered pathway of catecholaminergic fibers and the ectopic location of catecholaminergic neurons in this region.
Key words: catecholaminergic neuron; Pax6; netrin; proliferation; adhesion; axonal pathfinding
INTRODUCTION
Recently, a neuromeric model for catecholaminergic (CA) neuronal development has been proposed in several species, including lizard (Medina et al., 1994
), chick (Puelles and Medina, 1994
Gene expression studies have shown that the transcription factor Pax6 is transiently expressed in areas containing discrete CA neurons in the mesencephalon, the ventral thalamus, the hypothalamus (Stoykova and Gruss, 1994
In the present study, we first defined the localization of the Pax6 protein in CA [tyrosine hydroxylase-immunoreactive (TH-IR)] populations during development. We then investigated the role of Pax6 in these populations by looking at their development in mice lacking Pax6. We found that developing TH-IR neurons of the ventral thalamus [zona incerta (Zi)], hypothalamus (paraventricular nucleus), olfactory bulb, and basal telencephalon (anterior olfactory nucleus, piriform cortex, anterior amygdala, and olfactory tubercle) display high levels of Pax6 protein during a critical period of their development. Despite severe positional alterations, diencephalic and hypothalamic TH-IR neurons were identified in mice lacking Pax6, showing that Pax6 is not necessary for their specification. In contrast, TH-IR neurons were greatly reduced in number in the basal telencephalon and the remaining olfactory bulb. In addition, we found that ectopic TH-IR neurons were distributed ventrodorsally along the pretectal-dorsal thalamic transition zone and that TH-IR fibers were misguided in this zone and in the dorsal thalamic alar plate. Interestingly, this region displayed an increased and ectopic expression of the SHH-induced chemorepellant/chemoattractive molecule, Netrin-1 (Leonardo et al., 1997
MATERIALS AND METHODS
Animals. The original small-eye (Pax6sey) mutation arose spontaneously in a stock called "CSR" and was subsequently outcrossed. The genetic background of the small-eye strain used in this study was derived from the outbred Swiss background. The mating of Pax6sey/+ (small-eye heterozygotes) was confirmed by the presence of a vaginal plug the following morning. This was designated embryonic day 0.5 (E0.5). Experiments were performed on E11.5, E12.5, E13.5, E14.5, E16.5, E17.5, and E18.5 embryos. Embryos were dissected from deeply anesthetized mothers into cold PBS on ice and examined under a dissecting microscope. Homozygous Pax6sey/Pax6sey embryos were easily distinguished by their absence of eyes and characteristic craniofacial phenotype of foreshortened upper jaw. From E12.5, heterozygotes (Pax6sey/+) were distinguished by the characteristic appearance of their iris lacking its inferior margin (Kaufman et al., 1995
Immunocytochemistry. E11.5, E12.5, and E13.5 embryos were fixed by immersion in 4% paraformaldehyde in 0.1 M phosphate buffer (PB), pH 7.6. Embryos from E14.5 to E19.5 and postnatal mice were perfused transcardially with saline followed by 4% paraformaldehyde in PB. Whole embryos or brains were post-fixed for 2-5 d in the same fixative and cryoprotected in 30% sucrose in PB. Serial coronal or sagittal sections (40 µm) were cut on a freezing microtome and immediately processed for immunocytochemistry. In brief, sections were incubated with the primary antibodies diluted in PBS+ (0.1 M PBS with 0.2% gelatin and 0.25% Triton X-100) overnight at 4°C. Rabbit polyclonal anti-TH antibodies (1:8000, kind gift of A. Vigny, or 1:800, Protos Biotech), rabbit polyclonal anti-calretinin antibody (1:10,000: Swant), rabbit polyclonal anti-calbindin antibody (1:20,000; Swant), rat monoclonal anti-L1 antibody (1:50, Roche Diagnostics), and rat monoclonal anti-NCAM antibody (1:50; Roche Diagnostics) were used. Biotinylated goat anti-rabbit and biotinylated goat anti-rat (1:200, Dako, Glostrup, Denmark) were used as secondary antibodies and revealed with a streptavidin-biotin-peroxidase complex (1:200, Amersham, Buckinghamshire, UK). Sections were then reacted with a solution containing 0.02% diaminobenzidine, 0.6% nickel ammonium sulfate, and 0.003% H2O2 in 0.05 M Tris buffer, pH 7.6 (DAB-Ni). From these sections, the total number of TH-IR neurons in A14 paraventricular hypothalamic nucleus (PAVH) and the diameters of randomly selected TH-IR neurons (n = 20) were measured in A14PAVH from E17.5 wild-type (n = 4) and Pax6seyPax6sey (n = 4) embryos.
Double Pax6 and TH immunocytochemistry. Whole embryos (E11.5, E12.5, E14.5, E16.5, E17.5, and E18.5) and dissected postnatal (P0, P2, P4, and P9) and adult brains (5 and 16 weeks old) were immediately frozen in isopentane (
40°C) and stored at
Morphometric analysis. Free-floating sections (45 µm) were processed for TH immunocytochemistry as described above, except that immunolabeling was revealed using an FITC anti-rabbit antibody (1:200, Dako). Propidium iodide, a nuclear dye (1/10,000, Molecular Probes, Eugene, OR), was added during the last 10 min of incubation with the secondary antibody. Our analysis was performed on sections obtained from four wild-type and four Pax6sey/Pax6sey embryos. In each case, seven sections from wild-type embryos and five sections from Pax6sey/Pax6sey embryos taken through the Zi and the dorsomedial hypothalamic nucleus (DMH) were selected. By confocal microscopy (Leica), each section was resectioned into serial 7-µm-thick sections. To estimate the volume of A13 and A14DMH in wild-type and Pax6sey/Pax6sey embryos, the surface area of these nuclei in each section was measured using Leica TCNS software. For each brain, volumes were obtained by multiplying each area by the thickness of tissue between sections and summing the values. To estimate cell densities in A13 and A14DMH, the same sections were analyzed. In the areas defined by TH immunoreactivity, all propidium-labeled nuclei and all cells with a visible TH immunostaining were counted, and the averages of total cell density and of TH-IR neuronal density (per millimeter cubed) were calculated for each nucleus. From these sections, the diameters of randomly selected TH-IR neurons (n = 30) were measured in A13 and A14DMH in wild-type and Pax6sey/Pax6sey embryos using the same software.
Proliferation of tyrosine hydroxylase neurons. Pregnant mice were injected with a single dose of bromodeoxyuridine (BrdU; 25 mg/kg in sterile saline, i.p.) on E9.75, E10.5, E11.5, and E12.5 and were killed when embryos reached E17.5. Embryos were perfused transcardially with saline followed by 4% paraformaldehyde in PB, and brains were dissected, post-fixed overnight in the same fixative, and cryoprotected in 10% sucrose in PB. Brains were embedded in a solution containing 7% gelatin and 10% sucrose and frozen in isopentane. Alternate coronal sections (20 µm) were cut on a cryostat and processed for sequential immunolabeling. Half of the alternate sections were reacted for both TH and BrdU. Sections were first processed for TH immunocytochemistry as described above except that only DAB was used (0.03% DAB, 0.01% hydrogen peroxide in 0.1 M PBS). Then, sections were washed in TBS (0.09% NaCl, 50 mM Tris, pH 7.6), incubated for 8 min in 1 M HCl at 60°C, washed for 4 min with tap water, rinsed in TBS, incubated for 10 min in 20% rabbit serum in TBS, and finally incubated overnight with a solution containing mouse anti-BrdU (1:200, Becton-Dickinson) in 20% rabbit serum-TBS. Sections were washed in TBS, incubated for 2 hr with a biotinylated rabbit anti-mouse (1:200, Dako) in 20% rabbit serum-TBS, washed in TBS, incubated with a streptavidin-biotin-peroxidase complex (1:200, Amersham) for 2 hr at room temperature, and revealed with the DAB-Ni protocol (see above). The other half was Nissl-stained. To estimate the number of BrdU-labeled cells, a minimum of six sections taken through Zi and DMH were selected. On each section, A13 and A14DMH were identified, and the number of TH-IR neurons heavily labeled (defined as having >50% of the nucleus immunolabeled) for BrdU was estimated using 40× and 100× objectives. Only heavily labeled cells were counted because they would have been generated at the time of BrdU administration, whereas many lightly labeled cells would have been the products of further progenitor cell divisions (Gillies and Price, 1993
Nissl staining and counterstaining. Complete series of parasagittal and coronal paraffin sections (10 µm) obtained from E11.5, E12.5, E14.5, E16.5, and E18.5 wild-type and Pax6sey/Pax6sey embryos were Nissl-stained in a solution containing 0.05% thionin in acetic acid, pH 5.5.
In situ hybridization. E11.5, E12.5, E13.5, E14.5, E16.5, and E19.5 wild-type and Pax6sey/Pax6sey embryos were dissected in PBS, fixed, and cryoprotected overnight in 4% paraformaldehyde-30% sucrose. Sections (80-100 µm thick) were obtained on a freezing microtome, washed in PBS 0.1% Tween 20 (PTW), dehydrated for 20 min in methanol, and rehydrated in PTW before hybridization. Hybridization was performed as described in Henrique et al. (1995)
Nomenclature. On the basis of gene expression domains and anatomical features (constrictions in the neural wall and regions of low cell density), the brain has been subdivided into neuromeres. The rhombomeric and mesencephalic organizations have been described by Lumsden (1990)
RESULTS
Neuromeric location of TH-immunoreactive groups in E14.5 wild-type embryos
So far, no description of the neuromeric location of permanent and transient TH-IR groups is available in developing mice despite the increasing references to the neuromeric organization of the brain (Bulfone et al., 1993
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Figure 1. Determination of the neuromeric organization of TH-IR neurons in E14.5 wild-type embryos. Sagittal sections stained for Nissl (A) or immunoreacted for calbindin (B) or calretinin (C) have provided the prosomeric landmarks used for the determination of the segmental organization of TH-IR groups as shown in D-F. A, The section shows constrictions in the neural wall and regions of low cell densities associated with prosomeric boundaries. Arrowheads indicate, from caudal to rostral, the isthmic constriction, the caudal limit of the posterior commissure (PC) at the mesencephalic (mes)-p1 boundary, the fasciculus retroflexus (fr) at the p1-p2 boundary (in p2), and the stria medullaris (stm) at the p3-p4 boundary. The dotted line represents the angle used for coronal sectioning. B, Calbindin immunoreactivity shows the posterior commissure in the roof of p1, the nucleus of the posterior commissure (NPC) in p1, the dorsal thalamus (DT) in p2 alar plate, and thalamocortical axons (tc) running through p3 alar plate. The asterisk marks a strong immunoreactive hypothalamic region in p5 and p6 basal plate. The septum (SE) and olfactory bulb (OB) are also strongly immunoreactive. C, Calretinin immunoreactivity shows the posterior commissure, the subthalamic nucleus (Sut) in p4 basal plate, the thalamic eminence (EMT) in p4 alar plate, and the retrochiasmatic area (RCH) in p6 basal plate. The septum (SE) is also strongly immunolabeled. D-F, The prosomeric boundaries (continuous black lines) and basal-alar limit (dotted lines) are deduced from the adjacent sections stained for calretinin or calbindin. Note that B, C, and E are alternate sections. D, Medial section showing a subgroup of A11 organized along the fasciculus retroflexus and the A9-A10 complex. Note that A9 is located in the basal plate and extends from mes to p2, whereas A10 is located in the floor plate and extends from the isthmic (A10i) region to p3. E, A more lateral section than shown in D showing A11 extending from mes to p2 and the diencephalic and hypothalamic groups: A13 in p3, A14 in p4, and RCH and anterior preoptic (POA) areas in p6. F, A lateral section shows additional groups in the hypothalamus (A14 subgroups in p5 basal and alar plates) and in the telencephalon (A15). AB, Anterobasal nucleus; Is, isthmus; LGE, ganglionic eminence, lateral part; LL, lateral lemniscal area; MA, mammillary region; mes, mesencephalon; MGE, ganglionic eminence, medial part; mlf, medial longitudinal fasciculus; mtg, mammillotegmental tract; OR, optic recess; p1-p3, prosomeres; r1, rhombomere 1; SC, superior colliculus. Scale bar, A-F, 4 mm.
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Table 1. Mapping of the main TH-IR groups in E14.5 mouse brain Colocalization of Pax6 and TH immunoreactivities
TH-immunoreactive neurons displaying Pax6 immunoreactivity (Table 1)
Pax6 immunoreactivity was detected in three dopaminergic groups of the forebrain. In the alar plate of the ventral thalamus, a subpopulation (~40%) of TH-IR neurons of the zona incerta (A13) displayed a strong and transient Pax6 immunoreactivity from E12.5 to P9 (Fig. 2D,E). This subpopulation corresponds to the body of A13. In the hypothalamus, TH-IR neurons of the magnocellular part of the hypothalamic paraventricular nucleus displayed transient Pax6 immunoreactivity from E14.5 to P2 (A14PAVH in Table 1; data not shown). TH-IR neurons of the supraoptic nucleus (A15v) display also a transient Pax6 immunoreactivity from P0 to P9 (Table 1; data not shown). In the telencephalon, transient TH-IR neurons located in the anterior olfactory nucleus (A16AON) displayed Pax6 immunoreactivity from E14.5 to E18.5 (Table 1; data not shown). Transient TH-IR neurons of the piriform cortex, the olfactory tubercle, and the anterior amygdala display Pax6 immunoreactivity from E14.5 to E18.5 (Fig. 2 G-I). In the olfactory bulb (A16OB), TH-IR external tufted cells displayed Pax6 immunoreactivity from E14.5 and TH-IR periglomerular interneurons from E18.5 (Fig. 2J,K, Table 1).
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Figure 2. Pax6 protein expression in discrete developing TH-IR groups. Sections through the A8-A10 complex (A-C), the diencephalon and the hypothalamus (D-F), and the telencephalon (G-K) were double-immunostained with antibodies to TH (green; cytoplasmic staining) and Pax6 (red; nuclear staining). A-C, Absence of Pax6 and TH colocalization in the SN-VTA (A9-A10) complex and the retrorubral field (A8). A, The sagittal section shows a lack of Pax6 immunoreactivity in the developing SN-VTA of E12.5 embryo. Note the strong Pax6 immunolabeling of the deep mesencephalic nucleus (DPMe). B, The coronal section shows Pax6 immunoreactive cells (short arrows) in close proximity with TH-IR neurons of the dorsal part of the SN in E16.5 embryo. C, The coronal section shows Pax6 immunoreactive cells in the retrorubral field close to A8 neurons. D, The coronal section shows the colocalization of TH and Pax6 in A13 neurons of the zona incerta in the ventral thalamus. E, Higher magnification of the box shown in D showing individual double-immunolabeled cells (white arrows). Note the presence of TH-IR neurons (A13d) that do not express Pax6 (white arrow). F, The coronal section shows the lack of Pax6 immunoreactivity in A14DMH neurons of the hypothalamus. G, Coronal section showing Pax6-immunoreactive cells in the basal telencephalon. Pax6-immunoreactive cells are located in the anterior amygdala (large arrowhead) and the region of the piriform cortex (small arrowhead). Note Pax6 immunoreactive cells also in the cerebral cortex, hypothalamus, and ventral thalamus. H, Higher magnification of G showing individual double-labeled neurons at the level of the anterior amygdala. I, Higher magnification of G showing individual double-labeled neurons at the level of the piriform cortex (arrows). J, K, Coronal sections of the olfactory bulb. J, TH-IR external tufted cells display a strong Pax6 immunostaining in E15.5 embryo (small arrow). K, Both TH-IR periglomerular neurons and TH-IR external tufted cells in A16 display Pax6 immunoreactivity at P0. Scale bar: A, G, 6 mm; B, C, 4 mm; D, F, J, 1 mm; E, 0.25 mm; H, 0.12 mm; I, 0.5 mm; K, 5 mm.
TH-immunoreactive neurons not displaying Pax6 immunoreactivity (Table 1)
Noradrenergic (A1-A7) and adrenergic (C1-C3) neurons of the brainstem never displayed Pax6 immunoreactivity (Table 1). Dopaminergic neurons of the ventral tegmental area (A10i, A10m, A10p1, A10p2, and A10p3) in the floor plate, of the substantia nigra (A9m, A9p1, and A9p2), and of the retrorubral field (A8) in the basal plate, and of A11 complex (A11m, A11p1, A11p2) in the alar plate did not display Pax6 immunoreactivity throughout development (Fig. 2A-C). In the hypothalamus, the TH-IR groups listed below did not display Pax6 immunolabeling at any stage of development: the lateral hypothalamic nucleus (A14l), the medial preoptic area (POA and A14d), the arcuate nucleus (A12). In the telencephalon, TH-IR neurons of the bed nucleus of the stria terminalis (A15d) did not display Pax6 immunoreactivity. Although no colocalization of TH and Pax6 was observed in TH-IR neurons of the dorsal medial hypothalamic nucleus (Fig. 2F, A14DMH), Pax6 was expressed in the neuroepithelium of A14DMH during its period of genesis (from E9.75 to E12.5; see below).An overview of defects in Pax6sey/Pax6sey embryos
From E10.5 to E14.5, Pax6sey/Pax6sey embryos displayed a delay in their growth. A marked difference in their crown-rump length was observed at E11.5 (wild type: 4.8 ± 0.3 mm, n = 15; Pax6sey/Pax6sey: 3.8 ± 0.33 mm, n = 15). By E14.5, wild-type and Pax6sey/Pax6sey embryos displayed no significant difference in their crown-rump length (wild type: 11.7 ± 0.07 mm, n = 30; Pax6sey/Pax6sey: 11.1 ± 0.1 mm, n = 30). By E17.5, brain weights were similar in wild-type and Pax6sey/Pax6sey embryos (wild type: 0.76 ± 0.07 gm, n = 30; Pax6sey/Pax6sey: 0.74 ± 0.06 gm, n = 25). Some brain regions in Pax6sey/Pax6sey embryos have been shown to display higher than normal cell densities (Schmahl et al., 1993
TH-IR groups that did or did not display Pax6 immunoreactivity were described in Pax6sey/Pax6sey embryos within the same framework used above (see Fig. 3 for a general overview at E14.5). We observed several alterations in both Pax6-expressing TH-IR populations and TH-IR neurons that did not express Pax6, such as SN and VTA neurons. Noradrenergic (A1-A7) and adrenergic (C1-C3) neurons and mesencephalic dopaminergic neurons of A8, which did not express Pax6 (Table 1), displayed no delay and appeared normally organized in Pax6sey/Pax6sey embryos. The following description will focus on TH-IR groups displaying alterations.
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Figure 3. Determination of the presumptive neuromeric organization of TH-IR groups in E14.5 Pax6sey/Pax6sey embryos. Nissl-staining (A) and immunolabeling for calbindin (B) or calretinin (C) have provided prosomeric landmarks used for the determination of the segmental organization of TH-IR groups (D). A, The sagittal section shows constrictions in the neural wall and regions of low cell densities associated with neuromeric boundaries. From caudal to rostral, arrowheads point to the isthmic constriction and the presumptive, p1-p2, p2-p3, and p3-p4 boundaries. Thin arrows point to the presumptive p2-p3 and p3-p4 boundaries. Arrows point to the presumptive p1-p2, p2-p3, p3-p4, and p4-p5 boundaries. The dotted line represents the angle used for coronal sectioning. B, The sagittal section immunoreacted for calbindin shows a normal medial longitudinal fasciculus (mlf), retrochiasmatic (RCH) and anterobasal (AB) areas, and septum (SE). The white star indicates the lack of clustering of the presumptive dorsal thalamus and the lack of thalamocortical axons. C, Sagittal section immunoreacted for calretinin shows normal immunoreactivity in the thalamic eminence (EMT), the stria medullaris (sm), and the subthalamic nucleus (Sut) in p4. D, The sagittal section immunoreacted for TH shows numerous groups and complexes: A11, A9-A10, and in anterobasal and preoptic (POA) areas. The limit between mes and p1 is not indicated because this neuromeric limit is altered in the mutant (Mastick et al., 1997
Defects in Pax6-immunoreactive components of the incerto-hypothalamic axis
The incerto-hypothalamic axis (Bjorklund et al., 1975
Cell generation
In E11.5 wild-type embryos, it was possible to identify scattered TH-IR neurons in the ventral thalamus at the level of the primordium of A13 and a few medium-sized TH-IR neurons of the A14 complex in p4 and p5. These cells were more numerous by E12.5 (Fig. 4A). In Pax6sey/Pax6sey embryos, the A13 and A14 primordia appeared with a 2 d delay (Fig. 4A,B), and when they first appeared, they contained fewer TH-IR neurons than in wild-type embryos (50% reduction estimated). This delay did not persist. By E17.5, the total numbers of TH-IR profile counts in mutants and wild types were similar in A13 (n = 600 ± 65, from six wild types; n = 524 ± 60, from six mutants; values are means ± SEM), in A14DMH (n = 510 ± 40, from six wild types; n = 486 ± 60, from six mutants), and in A14PAVH (n = 40 ± 4, from four wild types; n = 38 ± 3, from four mutants). Because the mean diameters of TH-IR neuronal cell bodies were similar in wild-type (A13, n = 10 µm ± 0.7; A14DMH, n = 11 µm ± 0.7; A14PAVH, n = 12 µm ± 0.9; values are means ± SEM from 30 TH-IR neurons from four wild types) and Pax6sey/Pax6sey embryos (A13, n = 11 µm ± 0.6; A14DMH, n = 10.5 µm ± 1.0; A14PAVH, n = 11.5 µm ± 0.4, values are means ± SEM from 30 TH-IR neurons from four mutants), this indicates that there is no difference in TH-IR cell number in these structures.
Although Pax6 is expressed in differentiated TH-IR neurons of A13 and A14PAVH but not A14DMH, Pax6 is expressed during the time of genesis of all of these TH-IR populations. We have investigated a possible delay in cell generation of the cells destined for these groups in Pax6sey/Pax6sey embryos. Cell proliferation was studied by analyzing BrdU incorporation into S-phase cells and visualizing them at E17.5 using anti-BrdU and anti-TH antibodies (Fig. 4C-F). To identify the embryonic stages at which the neurons of these nuclei are generated, a single injection was applied at four different developmental stages: E9.75, E10.5, E11.5, and E12.5. The number of BrdU-TH-positive cells and TH-positive cells was determined on coronal sections at E17.5. The labeling index was calculated as the percentage of the total number of TH-positive cells that were BrdU-TH-positive. In wild-type embryos, A13 and A14DMH are generated from E9.75 to E11.5 with a peak at E10.5 (Fig. 4G,H, white bars). In Pax6sey/Pax6sey embryos, the labeling index after each injection was unchanged and no delay was observed (Fig. 4G,H, black bars), suggesting that cell generation is unaffected in A13 and A14DMH.
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Figure 4. Delay in the appearance of a TH phenotype in A13 and A14DMH is not caused by a cell proliferation defect. A, B, Sagittal sections of E12.5 wild-type (A) and Pax6sey/Pax6sey (B) embryos immunolabeled for TH. A, Arrow points to the A13 and A14 primordia. B, The black asterisk indicates the presumptive location of the A13 and A14 primordia in the mutant; note the lack of TH-IR neurons in these regions. C-F, Double immunolabeling for TH and BrdU of E17.5 wild-type (C, D) and Pax6sey/Pax6sey embryos (E, F) at the level of A13. BrdU was injected on E10.5. D, F, Arrows point to TH-BrdU double-labeled neurons. G, H, Histograms showing similar mean percentages (±SEM) of TH-IR neurons darkly labeled for BrdU in A13 (G) and A14DMH (H) in wild-type (white bars) and Pax6sey/Pax6sey (black bars) E17.5 embryos after injections of BrdU on E9.75-E12.5. Scale bar: A, B, 2 mm; C, E, 0.5 mm; D, F, 0.1 mm.
Positional alterations
In wild-type embryos, A13, A14DMH, and A14PAVH were populated by large TH-IR neurons and appeared fused with each other from E14.5 (Figs. 1F, 5A,C). In Pax6sey/Pax6sey embryos, A13, A14DMH, and A14PAVH appeared greatly disjoined and abnormally shaped (Fig. 5E-G). In wild-type embryos, three distinct A13 subgroups were observed from E16.5 (Hokfelt et al., 1984
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Figure 5. Alterations of the incerto-hypothalamic axis in E18.5 Pax6sey/Pax6sey embryos. Coronal sections are shown for wild-type (A-D) and Pax6sey/Pax6sey (E-H) embryos and are organized from caudal (top) to rostral (bottom). A-C, The components of the incerto-hypothalamic axis, A13, A14PAVH, and A14DMH appear fused together in wild-type embryos. The medial forebrain bundle is also indicated in A-D and F-H (large unlabeled arrows). A, Arrow indicates TH-IR neurons of the A14DMH complex. B, TH-IR neurons of A13 are divided into three distinct groups: a dorsal group (A13d), a lateral group (A13L), and a medial group A13 (A13). C, Arrow indicates TH-IR neurons of the paraventricular hypothalamic nucleus (A14PAVH). D, Rostral section at the level of the anterior commissure showing TH-IR neurons located in the medial preoptic nucleus (MnPo), the striato-hypothalamic nucleus (StHy), and the anterobasal region (AB). E-G, In Pax6sey/Pax6sey embryos, the components of the incerto-hypothalamic axis are completely disjoined and display abnormally high packing of the neurons. E, Arrows indicate A13 and A14DMH. Open arrows indicate abnormally located TH-IR fibers originating from the SN-VTA. F, Arrows indicate A13 and A14DMH. Projections from A14DMH to the area of the arcuate nucleus-median eminence are abnormally highly fasciculated. G, H, Arrows indicate the location of A14PAVH, StHy, the anterior medial preoptic nucleus (AMPo), MnPo, and AB. Scale bar: A-H, 2 mm.
Cellular segregation
In wild-type embryos, the structures of the incerto-hypothalamic axis, Zi, DMH, and PAVH are each composed of several neuronal groups with different phenotypes, such as TH, neurotensin, or vasopressin neurons. In these structures, TH-IR neurons are mixed with other cell types that do not express TH (Fig. 6A). In Pax6sey/Pax6sey embryos, TH-IR neurons constituting A13, A14DMH, and A14PAVH appeared more highly clustered (Fig. 6B). As described above, the total number of TH-IR neurons in A13, A14DMH, and A14PAVH are the same in the wild-type and Pax6sey/Pax6sey embryos (Fig. 6C-F); however, the volume occupied by A13 and A14DMH was smaller in Pax6sey/Pax6sey embryos (Fig. 6C). Interestingly, although the mean cellular density was similar between wild-type and Pax6sey/Pax6sey embryos (Fig. 6D), the cellular density of TH-IR neurons in these structures was higher in Pax6sey/Pax6sey embryos (Fig. 6F), indicating a higher segregation of TH-IR neurons in these structures as estimated by the increased percentage of TH-IR neurons within them (Fig. 6E). TH-IR neurons were more clustered or less mixed with cell types that did not express TH. This suggests altered adhesive properties of cells composing the Zi and DMH in Pax6sey/Pax6sey embryos.
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Figure 6. Increased cellular segregation of TH-IR neurons in A13 and A14DMH of mice lacking Pax6. TH was revealed with fluorescein-coupled antibodies (green in A and B), and nuclei were revealed on the same sections with propidium iodide (red in A and B). Pictures show the addition of two confocal images acquired simultaneously with a two-channel excitation beam. A, In A13 in the wild-type embryo, TH-IR neurons were mixed with non-TH-IR neurons. B, In Pax6sey/Pax6sey embryos, TH-IR neurons of A13 appeared more densely clustered and more segregated from the non-TH-IR neurons. C, Histogram shows the estimated volume occupied by TH-IR neurons in A14DMH and A13 in wild-type (white bars) and Pax6sey/Pax6sey (black bars) embryos. D, Histogram shows that the mean cell density of propidium-positive nuclei in A14DMH and A13 was similar in wild-type (white bars) and Pax6sey/Pax6sey (black bars) embryos. E, Histogram shows a significant increase of the percentage of TH-IR neurons compared with the total number of propidium-positive nuclei in A14DMH and A13 of Pax6sey/Pax6sey embryos. F, Histogram shows a significant increase in the density of TH-IR neurons in A14DMH and A13 in Pax6sey/Pax6sey embryos. C-F, Significant differences with Student's t test between groups are indicated: *p < 0.05; **p < 0.01. Scale bar: A, B, 0.75 mm.
Defects of TH-immunoreactive neurons in the telencephalon of Pax6sey/Pax6sey embryos
In wild-type embryos, from E14.5, TH-IR neurons were observed at the level of the bed nucleus (Fig. 7A, A15d) and the anterior olfactory nucleus (A16AON) (Nagatsu et al., 1990
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Figure 7. Defects of the telencephalic TH-IR neurons in Pax6sey/Pax6sey embryos. Coronal sections through the basal telencephalon and hypothalamus of E14.5 (A, C) and E18.5 (B, D) wild-type (A, B) and Pax6sey/Pax6sey (C, D) embryos. A, The section shows both the transient TH-IR neurons of the piriform cortex (pir) and the permanent TH-IR groups of A15v and A15d in continuation with A14d. Note the location of the medial forebrain bundle (mfb). B, High magnification of the pir-A15v area. C, The section shows a reduced A15d still in continuation with A14d. The black star indicates the lack of pir-A15v at the presumptive level of the rhinal fissure. D, The lack of pir-A15v persists in older age embryos (black star). The large asterisk indicates the abnormal swirl of TH-IR fibers at the medial forebrain bundle (mfb). Scale bar: A-E, 2 mm.
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Figure 8. Delay and diminution in the number of A16 neurons in the anterior olfactory nucleus and the residual olfactory structure of Pax6sey/Pax6sey embryos. Sagittal (A-C) and coronal (D-H) sections are shown for E14.5 (A-C, E-G) and E16.5 (D, H) wild-type (A-D) and Pax6sey/Pax6sey (E-H) embryos. Alternate sections are immunostained for calbindin (A, E), calretinin (B, F), or TH (C, F). A, Calbindin immunoreactivity labels short axon cells of the olfactory bulb. B, Calretinin immunoreactivity labels mitral and tufted cells of the olfactory bulb. C, Arrows indicate neurons of A16 in the anterior olfactory bulb in A16AON. D, Section showing TH-IR external tufted cells in the olfactory bulb of E16.5 wild-type embryo. E, Calbindin immunoreactivity strongly labels cells that may correspond to short axon cells. F, Calretinin immunoreactivity strongly labels cells that may correspond to the mitral and tufted cells of the remaining olfactory bulb. G, TH-IR neurons are absent in the remaining olfactory structure of E14.5 Pax6sey/Pax6sey embryo. E-G, Arrow points to the residual olfactory structure. H, High magnification shows scattered TH-IR neurons with short processes (arrows) in the residual olfactory bulb of E16.5 Pax6sey/Pax6sey embryo. Scale bar: A-C, E-G, 2 mm; D, H, 1 mm.
In wild-type embryos, from E16.5, TH-IR neurons were observed at the level of the strio-hypothalamic nuclei (Fig. 5D). In Pax6sey/Pax6sey embryos, despite the lack of the anterior commissure, TH-IR neurons were observed at the presumptive level of the strio-hypothalamic nucleus (Fig. 5H).
In addition, transient TH-IR neurons were observed in the piriform cortex (Fig. 7A,B, near A15v) from E14.5 to E18.5 and in the anterior amygdala (data not shown) and olfactory tubercle (data not shown) from E16.5 to E18.5 in wild-type embryos. In Pax6sey/Pax6sey embryos, TH-IR neurons were rare, round, and pale (n = 15 ± 4, values are mean ± SEM from four mutants; n = 90 ± 10, values are mean ± SEM from four wild types) at the presumptive level of the anterior amygdala. By E18.5, TH-IR neurons were not detected, and no pyknotic profiles were observed in this region. This suggests that these neurons were generated and had progressively lost their ability to maintain TH expression. TH-IR neurons were never observed in the presumptive olfactory tubercle, the piriform cortex (Fig. 7C,D), and the neighboring hypothalamic A15v (Fig. 7C) and at any age studied in Pax6sey/Pax6sey embryos.
Defects in TH-immunoreactive groups not expressing Pax6
Defects in the SN-VTA (A9-A10) and A11 complex
In wild-type embryos, from E11.5 to E13.5, TH-IR neurons of the primordium of the ventral tegmental area (A10i, A10m, A10p1, A10p2, and A10p3) and of the substantia nigra (A9m, A9p1, and A9p2) migrate radially from their proliferative zones to more superficial positions (Kawano et al., 1995
In wild-type embryos, the number of radially oriented TH-IR neurons detected in the vicinity of the ventricular surface gradually decreased by E13.5. By E14.5, most A9 and A10 neurons had reached their final locations in more superficial positions of the ventral floor plate and basal plate, respectively, and were oriented parallel to the ventral pial surface. From E16.5, TH-IR neurons of the A9 complex displayed their characteristic "inverted fountain" pattern (Hanaway et al., 1971
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Figure 9. Developmental defects of the SN-VTA complex in Pax6sey/Pax6sey embryos. A, Sagittal section showing the developing SN-VTA complex of E12.5 wild-type embryo. Arrowheads indicate the radially oriented TH-IR neurons from mes to p3. Note that TH-IR neurons of A10 in p3 (A10p3) display a less intense immunoreactivity. B, Coronal section of E18.5 wild-type embryo showing the characteristic topographical inverted fountain-like organization of the SN-VTA complex. C, D, Medial (C) and lateral (D) sagittal sections of E18.5 wild-type embryo showing the organization of the SN-VTA complex. E, Sagittal section of the developing SN-VTA complex in E12.5 Pax6sey/Pax6sey embryo showing the abnormal topographical organization of TH-IR neurons in p1 and p2 (small arrowheads). Small arrows point to A10p3; large arrowheads point to radially migrating TH-IR neurons. F, The coronal section shows the abnormal topographical organization of the SN-VTA complex in an E18.5 Pax6sey/Pax6sey embryo. B, F, Curved arrows emphasize the topographical organization of dopaminergic neurons of the SN and the main direction of their neuropils. G, H, Medial (G) and lateral (H) sagittal sections of E18.5 Pax6sey/Pax6sey embryo. The arrows point to TH-IR neurons abnormally located along the p1-p2 border and in p2. C, D, The black star indicates the lack of TH-IR neurons in wild-type embryo at the corresponding location where ectopic TH-IR neurons are seen in the mutant. Scale bar: A, E, 2 mm; B, F, 1 mm; C, D, G, H, 0.5 mm.
TH-IR fiber pathway alterations in Pax6sey/Pax6sey embryos
In wild-type embryos, by E11.5, nigrostriatal and mesocortical fibers originating from A9 and A10 followed the pathway of the medial forebrain bundle (mfb) in mes, p1, p2, p3, and p4 basal plate. By E14.5, nigrostriatal fibers terminated in the lateral portion of the caudate-putamen (Fig. 10A), whereas mesocortical fibers continued rostrally to reach the prefrontal cortex and the striatum by E15.5. In addition, a few TH-IR fibers originating from A10 were observed running along the fasciculus retroflexus toward the epithalamus (Skagerberg et al., 1984
In Pax6sey/Pax6sey embryos, by E11.5, most TH-IR fibers did not follow the pathway of mfb. Fibers were misguided along the presumptive p1-p2 transition zone where they followed a straight ventrodorsal course (Fig. 10B,C). A few fibers originating from the more rostral and ventromedial neurons of the A9-A10 complex followed the pathway of the presumptive mfb (Fig. 10D), although they only reached p4 by E12.5. By E14.5, misguided TH-IR fibers looped in the roof of p2, plunged mediolaterally after the presumptive p2-p3 border, and turned rostroventrally in p3 basal plate to reach and follow the pathway of the presumptive mfb in p4 and p5 (Fig. 10E-J). In addition, few TH-IR fibers looped rostrally in presumptive p2 alar plate (Fig. 10E,G). In their ascending and descending courses, TH-IR fibers appeared abnormally highly fasciculated (Fig. 10H). At the presumptive level of the internal capsule and the optic tract, TH-IR fibers swirled just before they entered the caudate putamen (Fig. 7D). From E18.5, at least some TH-IR fibers reached the same rostral levels as observed in wild-type embryos, although the number of terminals was greatly reduced, particularly in the olfactory tubercle (Fig. 10L).
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Figure 10. Alterations of TH-IR fibers pathway in Pax6sey/Pax6sey embryos. Sagittal (A-J) and coronal (K, L) sections are shown for wild-type (A, K) and Pax6sey/Pax6sey (B-J, L) embryos. Embryos were sectioned at E11.5 (B-D), E14.5 (A, E-J), and E18.5 (K, L). Large arrows indicate the direction of the fibers. A, Large arrow indicates the direction of the medial forebrain bundle (mfb), the major fiber pathway originating from TH-IR neurons of the SN-VTA complex. B, The sagittal section shows early alterations of TH-IR fiber pathway. C, D, Small arrowheads point to growth cones. C, Higher magnification of area outlined in B, showing that most of the TH-IR fibers are abnormally deflected dorsally after the presumptive pretectal-dorsal thalamic boundary. D, Higher magnification of area outlined in B shows that some TH-IR fibers are not deflected dorsally. E, A lateral section shows a high number of fibers from the SN-VTA complex misguided in the diencephalic alar plate (arrow). F, A mediolateral section of Pax6sey/Pax6sey embryos indicating neurons of the SN and their projections. Arrow indicates some TH-IR neurons of the SN that are not misguided. G, A medial section shows TH-IR fibers looping in the roof of the diencephalon (arrow). H, I, J, Higher magnifications of E, G, and F, respectively. H, Reconstruction of TH-IR fiber pathway. K, The coronal section shows the main projecting areas of TH-IR fibers, the striatum (ST), the nucleus accumbens (ACB), and the olfactory tubercle (OT). L, TH-IR fibers terminated normally in the striatum and the nucleus accumbens of Pax6sey/Pax6seyembryo. The black star indicates a lack of terminals in the olfactory tubercle. Scale bar: A, E-G, K, J, 4 mm; B, 2 mm; C, H-J, 1 mm; D, 0.5 mm.
General fiber pathway alterations in Pax6sey/Pax6sey embryos
Using the neuronal cell adhesion molecules NCAM and L1 as general markers of most axonal pathways, we analyzed whether alterations of TH-IR axons in the presumptive diencephalon were a selective defect of catecholaminergic fibers or a general defect of all ascending and descending fibers.
NCAM (from E11.5 to E13.5) and L1 (from E14.5) immunoreactivities revealed most of the fiber pathways traveling in the diencephalon. In wild-type embryos, the posterior, pretectal, and tectal commissures, the fasciculus retroflexus, and the stria medullaris were labeled with NCAM (Fig. 11B) or L1 (Fig. 11E). In addition, the zona limitans intrathalamica (Zli) at the p2-p3 boundary displayed NCAM immunoreactivity from E11.5 to E13.5 (Fig. 11B).
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Figure 11. Alterations of specific fiber pathways in Pax6sey/Pax6seyembryos. Sagittal sections are shown for E12.5 wild-type (A, B) and Pax6sey/Pax6sey (C, D) embryos. Nissl-stained sections (A, C) are shown in parallel with sections immunoreacted for NCAM (B, D). A, C, The sagittal section shows constrictions and regions of low cell densities associated with prosomeric boundaries. A, C, Arrows indicate, from caudal to rostral, the mes-p1 boundary and the p1-p2 boundary. B, NCAM immunoreactivity reveals ascending and descending fibers of the posterior commissure (pc), the fasciculus retroflexus (fr), the stria medullaris (sm), and thalamic axons. A cellular labeling also reveals the zona limitans intrathalamica (zli). D, A remaining pc is distinguishable in p1 but most of the fiber tracts are misguided in the diencephalon (white arrowhead). E, F, Sagittal sections immunoreacted for L1 are shown for E18.5 (E), wild-type, and (F) Pax6sey/Pax6sey embryos. E, The sagittal section shows the posterior commissure (pc) in the caudal part of the pretectum and the fasciculus retroflexus (fr) at the pretectal-dorsal thalamic transition zone. F, The sagittal section shows aberrant fiber pathways in the pretectal and dorsal thalamic alar plate (between the arrows). Note that fibers traveling in the lower part of the basal plate and in the floor plate maintain a normal trajectory. Scale bar: A-D, 4 mm; E, F, 8 mm.
In Pax6sey/Pax6seyembryos, fibers traveling medially followed a normal trajectory in the basal plate of the rhombencephalon, mes, p1, p2, and p3, whereas fibers located laterally in basal plate and alar plate were misguided at the presumptive p1-p2 transition zone and in p2 alar plate (Fig. 11D,F). In p2, most of the L1 immunoreactive fibers were highly fasciculated into several straight and parallel bundles (Fig. 11F). In the roof of p2, most fibers looped and descended at the presumptive p2-p3 limit.
Altered expression of the chemorepellent/chemoattractive molecule Netrin-1 in Pax6sey/Pax6sey embryos
In Pax6sey/Pax6sey embryos, from E11.5, the developmental expression of Netrin-1 was roughly normal in the rhombencephalic and mesencephalic floor plate, along the floor of the fourth ventricle and along the wall of the lateral ventricle (Fig. 12). From E13.5, Netrin-1 was normally expressed in the striatum and from E14.5 in the vicinity of the SN-VTA complex (Livesey and Hunt, 1997
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Figure 12. Alteration of Netrin-1 expression in the diencephalon of Pax6sey/Pax6sey embryos. Coronal (A, C) and sagittal (B, D) sections of E14.5 (B, D) and E16.5 (A, C) wild-type (A, B) and Pax6sey/Pax6sey (C, D) embryos. A, In the mesencephalon, Netrin-1 is expressed at the level of the SN-VTA complex. B, The sagittal section shows Netrin-1 expression in the floor of the fourth ventricle and in the basal plate of p1, p2, and p3. Note also a weak expression along the zona limitans intrathalamica (Zli). C, The coronal section shows a normal Netrin-1 expression at the level of the SN-VTA complex. D, In the diencephalon, Netrin-1 expression is increased and expanded dorsally. Arrows indicate the dorsal expansion in the ventral and dorsal thalamic alar plates. mes, Mesencephalon. Scale bar: A, C, 4 mm; B, D, 2 mm.
DISCUSSION
Our results in normal mice are in good agreement with previous comparative analyses on catecholaminergic systems in sauropsides (Medina et al., 1994
It has been suggested that Pax6 could be a good candidate for controlling the proliferation, specification, or maintenance of discrete CA populations (Stoykova and Gruss, 1994
Dopaminergic populations expressing Pax6
Diencephalic and hypothalamic TH-IR neurons: cell adhesion defect
The neuroepithelium of prosomeres 3, 4, and 5 expresses Pax6 during the time of genesis of diencephalic and hypothalamic TH-IR neurons. Our study indicates that differentiated TH-IR neurons of A13 and A14PAVH continue to express Pax6 until the first postnatal days, whereas A14DMH does not. In mice lacking Pax6, these populations differentiate but display a 1-2 d delay in their appearance. Because previous studies have shown abnormally low proliferative rates in the entire diencephalic alar plate of mice lacking Pax6 (Warren and Price, 1997Telencephalic populations: cell migration/maintenance defect
In the olfactory bulb, Pax6 is expressed from E15.5 in TH-IR external tufted cells and from E18.5 in TH-IR periglomerular interneurons. In mice, external tufted cells are born between E13 and E18 (Hinds, 1968aDefects in catecholaminergic populations not expressing Pax6
Although TH-IR neurons of the SN-VTA complex never display Pax6 immunoreactivity, we show in mice lacking Pax6 an abnormal location of TH-IR neurons and an alte
