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Progress in Neurobiology 64 (2001) 69 – 95 www.elsevier.com/locate/pneurobio Otx genes in brain morphogenesis Dario Acampora a,b, Massimo Gulisano c, Vania Broccoli d, Antonio Simeone a,b,* b a International Institute of Genetics and Biophysics, CNR, Via G. Marconi 12, 80125 Naples, Italy MRC Centre for De6elopmental Neurobiology, 4th Floor, King’s College London, Guy’s Campus, New Hunts House, London Bridge, London SE1 9RT, UK c Department of Physiological Sciences, Uni6ersity of Catania, Viale A. Doria 6, 95125 Catania, Italy d TIGEM-Telethon Institute of Genetics and Medicine, H.S. Raffaele Via Olgettina 58, 20132 Milan, Italy Received 30 May 2000 Abstract Most of the gene candidates for the control of developmental programmes that underlie brain morphogenesis in vertebrates are the homologues of Drosophila genes coding for signalling molecules or transcription factors. Among these, the orthodenticle group includes the Drosophila orthodenticle (otd) and the vertebrate Otx1 and Otx2 genes, which are mostly involved in fundamental processes of anterior neural patterning. These genes encode transcription factors that recognise specific target sequences through the DNA binding properties of the homeodomain. In Drosophila, mutations of otd cause the loss of the anteriormost head neuromere where the gene is transcribed, suggesting that it may act as a segmentation ‘gap’ gene. In mouse embryos, the expression patterns of Otx1 and Otx2 have shown a remarkable similarity with the Drosophila counterpart. This suggested that they could be part of a conserved control system operating in the brain and different from that coded by the HOX complexes controlling the hindbrain and spinal cord. To verify this hypothesis a series of mouse models have been generated in which the functions of the murine genes were: (i) fully inactivated, (ii) replaced with each others, (iii) replaced with the Drosophila otd gene. Otx1−/− mutants suffer from epilepsy and are affected by neurological, hormonal, and sense organ defects. Otx2− /− mice are embryonically lethal, they show gastrulation impairments and fail in specifying anterior neural plate. Analysis of the Otx1−/−; Otx2+/− double mutants has shown that a minimal threshold level of the proteins they encode is required for the correct positioning of the midbrain-hindbrain boundary (MHB). In vivo otd/Otx reciprocal gene replacement experiments have provided evidence of a general functional equivalence among otd, Otx1 and Otx2 in fly and mouse. Altogether these data highlight a crucial role for the Otx genes in specification, regionalization and terminal differentiation of rostral central nervous system (CNS) and lead to hypothesize that modification of their regulatory control may have influenced morphogenesis and evolution of the brain. © 2001 Elsevier Science Ltd. All rights reserved. Contents 1. Introduction . . . . . . . . . . . . . . . . . . . . . . . . . 2. Multiple roles of the Otx1 gene in the developing and 2.1. Otx1 expression in early embryogenesis . . . . . 2.2. Otx1 expression during corticogenesis. . . . . . . . . . . . . . . adult mouse . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 70 71 71 71 Abbre6iations: ame, axial mesendoderm; AML, anterior midline; A/P, antero-posterior; AVE, anterior visceral endoderm; b-FSH, follicle-stimulating hormone; a-GSU, a-glycoprotein subunit; b-LH, luteinizing hormone; BrdU, Bromodeoxyuridine; CDGA, constitutional delay in growth and abdolescence; CNS, central nervous system; CP, cortical plate; d.p.c., days post coitum; D/V, dorso-ventral; EEG, electroencephalographic recording; EPSP, excitatory post-synaptic potentials; GABA, g-aminobutyric acid; GH, growth hormone; GnRH, gonadotropin releasing hormone; GnRHR, gonadotropin releasing hormone receptor; GRH, growth hormone releasing hormone; GRHR, growth hormone releasing hormone receptor; IGF1, insulin growth factor 1; IPSP, inhibitory post-synaptic potentials; IsO, isthmic organizer; IZ, intermediate zone; MHB, midbrain-hindbrain boundary; otd, Drosophila orthodenticle; RA, retinoic acid; VE, visceral endoderm; VZ, ventricular zone; ZLI, zona limitans intrathalamica. * Corresponding author. Tel.: +44-20-78486536; fax: +44-20-78486550. E-mail address: [email protected] (A. Simeone). 0301-0082/01/$ - see front matter © 2001 Elsevier Science Ltd. All rights reserved. PII: S0301-0082(00)00042-3 D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 70 2.3. 2.4. 2.5. 2.6. 2.7. Otx1 is required for correct brain development . . . . . . . . . Otx1−/− mutant mice exhibit an epileptic phenotype . . . . Otx1 controls cortical connectivity to subcortical targets. . . . Otx1 transiently controls GH, FSH, and LH in the pituitary . Otx1 is necessary for correct sense organ development . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 3. Early requirement of Otx2 for normal gastrulation and anterior neural plate induction and maintenance . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 3.1. Organisers and molecules in the current scenario of the anterior brain patterning . . . 3.2. Specification of anterior patterning requires Otx2 function . . . . . . . . . . . . . . . . 3.3. The role of Otx2 in the induction and maintenance of rostral CNS identities . . . . . 3.4. AVE-restricted OTX2 function is necessary for proper expression of Lim1 and bone morphogenetic protein (BMP) antagonists in the ame . . . . . . . . . . . . . . 3.5. Specific and interchangeable roles between Otx1 and Otx2 . . . . . . . . . . . . . . . . 71 72 73 73 73 74 74 75 78 79 80 4. Brain patterning depends on a critical Otx gene dosage . . . . . . . . . . . . . . . . . . . . . 4.1. Morphogenetic origin of the IsO . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 4.2. Otx genes are required for correct positioning of the isthmus . . . . . . . . . . . . . . . 80 80 81 5. otd/Otx conserved functions throughout evolution. . . . . 5.1. Otx genes in the animal kingdom . . . . . . . . . . . 5.2. A common genetic program in insect and vertebrate 5.3. Otx genes in brain evolution . . . . . . . . . . . . . . . . . . 85 85 87 89 6. Conclusions . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 90 Acknowledgements . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 90 References . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . 91 1. Introduction The central nervous system (CNS) of vertebrates is a very complex structure derived from a multistep process involving sequential molecular and morphogenetic events that pattern the epiblast first and the neural plate later. During early gastrulation the concerted and sequential action of both the anterior visceral endoderm (AVE) and the node-derived axial mesendoderm (ame, Beddington and Robertson, 1999; Bachiller et al., 2000) drives the specification of anterior neuroectoderm that, later on results grossly subdivided in three main territories (forebrain, midbrain and hindbrain, Gallera, 1971; Storey et al., 1992; Ruiz i Altaba, 1994; Shimamura and Rubenstein, 1997; Rubenstein and Beachy, 1998). The maintenance of this patterning is likely dependent on signals originating from the ame and/or within the overlying neuroectoderm (Acampora et al., 1998b; Rhinn et al., 1998; Shawlot et al., 1999; Camus et al., 2000). Anatomical and histological studies postulate the existence of genetic fate determinants which subdivide these large neural regions into progressively smaller longitudinal and transverse domains (Vaage, 1969; Altman and Bayer, 1988; Figdor and Stern, 1993; Rubenstein et al., 1994). Some of the patterning events along the antero-posterior (A/P) axis require the presence of . . . . . . . . . . . . . . . . . . . . . . head development . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . . specific cell populations (e.g. the anterior neural ridge and the zona limitans intrathalamica (ZLI)) and transverse rings of neuroepithelia (e.g. the isthmic organizer (IsO)) that possess inductive and boundary properties (Marin and Puelles, 1994; Crossley et al., 1996; Houart et al., 1998; Rubenstein et al., 1998; Ruiz i Altaba, 1998). In vertebrates, several genes controlling developmental programmes underlying brain morphogenesis have been isolated and their role studied in detail. Most of them are the vertebrate homologues of Drosophila genes encoding signalling molecules or transcription factors (Lemaire and Kodjabachian, 1996; Tam and Behringer, 1997; Rubenstein et al., 1998). Among these, the orthodenticle group is strictly defined by the Drosophila orthodenticle (otd) and the vertebrate Otx1 and Otx2 genes, which contain a bicoid-like homeodomain (Finkelstein and Boncinelli, 1994; Simeone, 1998). However, other genes that might be more distantly related to otd/Otx genes have been also identified (Muccielli et al., 1996; Szeto et al., 1996; Chen et al., 1997). Expression pattern analysis of Otx genes had suggested that these transcription factors might play an important role during brain morphogenesis in vertebrates. A systematic genetic approach using transgenic mice is revealing that they contribute to the molecular mechanisms underlying all of the major events (induc- D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 tion, maintenance, regionalization, corticogenesis and axon connectivity) necessary to build a normal brain. 2. Multiple roles of the Otx1 gene in the developing and adult mouse 2.1. Otx1 expression in early embryogenesis Otx1 starts to be expressed at early stages (2–5 somite stage, 8.2 –8.5 days post coitum (d.p.c.)) in the developing mouse embryo throughout the presumptive forebrain and midbrain neuroepithelium (Simeone et al., 1992). From these stages onwards its expression largely overlaps with that of Otx2, but while the expression of the latter disappears from the dorsal telencephalon since 10.5 d.p.c. (Simeone et al., 1993), Otx1 expression is maintained uniformly across the ventricular zone (VZ) of the cortical anlage from the onset of corticogenesis up to mid- to late gestation stages (Simeone et al., 1993; Frantz et al., 1994). Otx1 is also expressed at early stages in precursor structures of sense organs corresponding to the olfactory placode, otic and optic vesicles (Simeone et al., 1993). Later on, Otx1 is transcribed in the olfactory epithelium, the saccule, the cochlea and the lateral semicircular canal of the inner ear as well as in the iris, the ciliary process in the eye and the lachrymal gland primordia (Simeone et al., 1993). From the birthday onwards, Otx1 is also expressed at a relatively low level in the anterior lobe of the pituitary gland (Acampora et al., 1998c). 2.2. Otx1 expression during corticogenesis The cerebral cortex develops according to molecular strategies that determine the fate of precursor cells linked to specific neuronal phenotypes. Two main processes have been identified so far, laminar determination, by which committed cells migrate to their appropriate layer, and cortical areas formation, by which cortical neurons interact to create functionally distinct regions. During corticogenesis, postmitotic neurons migrate along radial glial cells (Rakic, 1972), through the overlying intermediate zone (IZ), and to the cortical plate (CP), which will later create the typical layered organisation of the adult cortex. The layers are generated in an inside-out pattern, in which cells of the deepest layers (6 and 5) are born first in the VZ, and those of the upper layers (4, 3, and 2) progressively later (Rakic, 1974). Otx1 represents a molecular correlate of deep layer neurogenesis and its expression is confined to neurons of layers 5 and 6 in the adult cortex (Frantz et al., 1994). 71 At mid-late gestation, high level transcription of Otx1 occurs only in ventricular cells, which at these stages are precursors of deep layer neurons. By the time upper layer neurons are generated, Otx1 expression decreases in the VZ and becomes progressively prominent in the cortical plate which consists of postmigratory neurons of layer 5 and 6. Otx1 is absent in later differentiated neurons of upper layers 1–4 (Frantz et al., 1994). Thus, the progressive down-regulation of Otx1 in the ventricular cells suggests that Otx1 may confer deeplayer identity to young neurons. Heterochronic transplantation experiments have demonstrated that the broad differentiative potentials of the early progenitors (McConnell and Kaznowski, 1991) become progressively restricted over time (Frantz and McConnell, 1996). Indeed, Otx1 expression is heterogeneous across the regions of the adult cortex, suggesting that it might also be involved in the forming of the cortical areas. Its expression in layer 5 is more prominent in the posterior and lateral cortex but absent in the frontal, insular and orbital cortices, while in layer 6 it is more uniform throughout the neocortex (Frantz et al., 1994). Mouse mutant models have been generated and analysed (Acampora et al., 1996, 1998a, 1999a,b Suda et al., 1996; Morsli et al., 1999; Weimann et al., 1999; Avanzini et al., submitted) to gain insight into the different roles that Otx1 plays during brain, cortex and sense organ development. 2.3. Otx1 is required for correct brain de6elopment Heterozygous (Otx1 + /−) mice are healthy and their intercross generates homozygous mice (Otx1−/ − ) in the expected mendelian ratio. However, about 30% of the mutants die before the first postnatal month, and appear smaller in size.Table 1 Otx1− /− adult brains are reduced in weight and size and, at the anatomo-histological inspection, show reduction in thickness of the dorsal telencephalic cortex, a dorsally displaced sulcus rhinalis and shrunken hippocampus with a divaricated dentate gyrus. The cortex is particularly affected at the level of the temporal and perirhinal areas, where a 40% reduction in cell number is detected. Furthermore, in these same areas, cortical layer organisation is less evident (Acampora et al., 1996), although the expression of layer-specific molecular markers demonstrates that the laminar identities are preserved (Weimann et al., 1999). The origin of the overall reduction of the Otx1−/− brains has been investigated through experiments aimed at determining possible changes of the normal number of apoptotic or proliferating cells within the neuroepithelium of the developing telencephalon. No differences at apoptosis were observed by comparing D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 72 wild-type and Otx1 mutant embryos. By contrast, Bromodeoxyuridine (BrdU) labelling experiments revealed a reduction of proliferating cells (by about 25%) in the dorsal telencephalic neuroepithelium of 9.75 d.p.c. Otx1−/− embryos (Acampora et al., 1998a). A defective proliferation of neuronal progenitors at these early stages may thus be responsible of the adult phenotype of the Otx1 mutant mice. 2.4. Otx1 −/− mutant mice exhibit an epileptic phenotype Otx1−/− mice exhibit both spontaneous high speed turning behaviour and epileptic behaviour (Acampora et al., 1996). The latter consists of the combination of, (i) focal seizures characterised by automatisms (head bobbing and teeth chattering) and electroencefalographic (EEG) recording of spikes in hippocampus; (ii) generalised seizures characterised by convulsions and high voltage synchronised EEG activ- ity in hippocampus and cortex. Occasionally, convulsions are followed by status epilepticus and exitus. Recently, the epileptogenic mechanisms accounting for these seizures have been further investigated by means of electrophysiological recordings (current clump intracellular recordings) made from layer 5 pyramidal neurons in somatosensory cortical slices (Avanzini et al., 2000). This analysis shows that g-aminobutyric acid (GABA)-mediated inhibitory post-synaptic potentials (IPSP), as compared with control pyramidal neurons, are more pronounced in the mutants where they seem to be involved in the synchronisation of the excitatory activity from the earliest postnatal period. On the other hand, multisynaptic excitatory post-synaptic potentials (EPSP) are significantly more expressed in the mutants than in controls, also at the end of the first postnatal month. These results suggest that the excessive excitatory amino acid-mediated synaptic driving, without a well-developed GABA counteraction, may lead to a hyperexcitable condition that is responsible for the epileptic manifestations occurring in Otx1 − /− mice. Table 1 Major phenotypes observed in Otxl−/−; hOtx21/hOtx21 and otd1/otd1 mutant mice Major phenotypes Otx1−/− hOtx21/hOtx21 otd 1/otd 1 Dorsal telencephalon Cell proliferation rate at E9.75 At E 13.5 and E 15.5 Reduced by 25% Reduced by 10% Full recovery Full recovery Full recovery Full recovery Cerebral cortex Cell number Layer organisation Laminar fatea Temporal cortex Perirhinal cortex Hippocampus Reduced Altered Normal Reduced by 40% Reduced by 40% Shrunken Full recovery Full recovery N/Ab Full recovery Full recovery Full recovery Full recovery Full recovery N/Ab Full recovery Full recovery Full recovery Mesencephalon Size of colliculi Enlarged Identities of colliculia Cerebellum Normal Abnormal foliation Normal in 15% Intennediate in 50% N/Ab Recovery in 10% Axonal projection from layer 5 neurons of 6isual cortex a Defective refinement of exuberant projections Normal in 30% Intermediate in 45% N/Ab Recovery in 50% N/Ab Beha6iour Turning behaviour Epileptic seizures High-speed Present Moderate-speed Absent Moderate-speed Absent Pituitary gland Impaired Normal Normal Ear Lateral semicircular duct Absent Absent Absent Eye Iris Reduced Recovery in 80% Ciliary process Lachrymal and Harderian gland Absent Absent Recovery in 80% Present in 70% Present in 75% a b Data from Weimann et al. (1999). N/A, not analysed. N/Ab Present in 80% Present in 34% D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 2.5. Otx1 controls cortical connecti6ity to subcortical targets Recent analysis of axonal projections in Otx1 − /− mutants has shed new light on the role of Otx1 during brain development (Weimann et al., 1999). In several brain regions, connections usually develop by a biphasic mechanism in which an excess of early formed axon projections is finely pruned by elimination of inappropriate axon terminals. Layer 5 neurons in the visual cortex provide a good example of exuberance in connectivity, establishing, among others (e.g. to corpus callosum), connections to a number of subcortical targets such as the pons, superior and inferior colliculi, and spinal cord. During early postnatal life, they selectively eliminate connections from the inferior colliculus and spinal cord (Stanfield and O’Leary, 1985; Stanfield et al., 1982), but the molecular mechanisms underlying this remodelling are poorly understood. Otx1 is strongly expressed in a subset of layer 5 neurons that form subcortical but not cortical connections (Weimann et al., 1999) and in layer 6 neurons, many of which forming thalamic projections. Analysis of Otx1−/− mutants reveals significant defects, specifically in the patterning of subcortical projections. In fact, while callosal and thalamic projections appear normal in the Otx1−/ − mutants, there are additional extensive innervations of both the inferior colliculus and the spinal cord that have been erroneously maintained. This phenotype suggests that Otx1 function is required for the last step of subcortical axon development, in which exuberant connections undergo extensive refinement with the elimination of axon projections from inappropriate targets (Weimann et al., 1999). 2.6. Otx1 transiently controls GH, FSH, and LH in the pituitary Otx1 is postnatally transcribed and translated in the pituitary gland. Cell culture experiments indicate that Otx1 may activate transcription of the growth hormone (GH), follicle-stimulating hormone (b-FSH), luteinizing hormone (b-LH), and a-glycoprotein subunit (a-GSU) genes. Analysis of Otx1 null mice (Acampora et al., 1998c) indicates that, at the prepubescent stage, they exhibit transient dwarfism and hypogonadism due to low levels of pituitary GH, FSH and LH hormones which, in turn, dramatically affect downstream molecular and organ targets. Nevertheless, Otx1 −/ − mice gradually recover from most of these abnormalities, showing normal levels of pituitary hormones with restored growth and gonadal function at 4 months of age. Expression patterns of related hypothalamic genes such as the growth hormone releasing hormone (GRH), gonadotropin releasing hormone (GnRH), and their pituitary receptors (GRHR and GnRHR) suggest that, 73 in Otx1− /− mice, hypothalamic and pituitary cells of the somatotropic and gonadotropic lineages appear unaltered and that it is the ability to synthesise GH, FSH, and LH, rather than the number of cells producing these hormones, to be affected (Acampora et al., 1998c). An intriguing aspect of our observation is the fact that transcription factors of the Ptx and Otx subfamilies recognise similar DNA target sequences (Simeone et al., 1993; Lamonerie et al., 1996; Szeto et al., 1996; Tremblay et al., 1998), and that Ptx1 and Ptx2 are expressed in most pituitary lineages, in particular in somatotrophic and gonadotrophic cells (Tremblay et al., 1998). Ptx1 is the most highly expressed of these genes, followed by Ptx2 and then Otx1 (Tremblay et al., 1998). Yet, the Otx1 knock-out has a dramatic effect only during the prepuberal period. The unique activity of Otx1 during this period might reflect a specific interaction of Otx1, but not of the related Ptx factor(s), with a transcription co-regulator in the somatotrophic and gonadotrophic cells. Taken together with previous reports, our observations support the existence of complex regulatory mechanisms defining combinatorial cell- and stage-specific interactions between transcription factors belonging to the same or to different gene families for the establishment/maintenance of pituitary function. A novel feature of this phenotype is the fact that most of the impaired functions are recovered by the adult stage. Indeed, after the prepubescent stage, Otx1 mutant mice begin to gradually recover from their abnormalities, showing at 4 months of age normal levels of GH, FSH and LH which are paralleled by a restored normal body weight, differentiation and size of both testis and ovary, as confirmed also by their sexual fertility, and by normal levels of downstream molecular targets such as testosterone and insulin growth factor 1 (IGF1). Although we are unable to explain the mechanism underlying this recovery, this observation might represent a possible example of temporal-restricted competence in hormonal regulation of specific cell-lineages by the Otx1 transcription factor. This recovery appears similar to the ‘catch-up growth’ (Boersma and Wit, 1997) described in children with delayed growth and puberty, also called ‘constitutional delay in growth and abdolescence’, CDGA (Horner et al., 1978). 2.7. Otx1 is necessary for correct sense organ de6elopment Otx1− /− mutants show inner ear and eye abnormalities that are consistent with Otx1 expression pattern (Acampora et al., 1996). Otx1 is expressed in the lateral canal and ampulla as well as in a part of the utricle, in the saccule and cochlea. Interestingly, Otx2 is co-expressed with Otx1 74 D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 in the saccule and cochlea but not in the components of the pars superior. Lack of Otx1 results in the absence of the lateral semicircular canal and lateral ampulla, in abnormal utriculosaccular and cochleosaccular ducts and in a poorly defined hook (the proximal part) of the cochlea (Acampora et al., 1996; Morsli et al., 1999). Defects in the shape of the saccule and cochlea are variable in Otx1 −/ − mice and are much more severe in Otx1− /−; Otx2 +/ − background. In Otx1 − /− and Otx1 −/−; Otx2 +/ − mutants the lateral crista is absent and the maculae of the utricle and saccule are partially fused (Morsli et al., 1999). In the eye and annexed structures Otx1 transcripts are restricted to the iris, ciliary process and ectodermal cells migrating from the eyelid and included in the mesenchymal component of the lachrymal glands. These ectodermal cells are believed to induce differentiation of the mesenchymal cells into a glandular exocrine cell-type. In Otx1 −/ − mice the ciliary process is absent, the iris is thinner and the lachrymal and Harderian glands do not develop, failing the differentiation to a glandular cell-type. Interestingly, the ectodermal cells embedded within the mesenchymal components are not identified in Otx1 −/ − mice, thus indicating that failure in development of the glands is a consequence of the impaired migration of the ectodermal cells from the eyelid to the mesenchyme of the lachrymal primordium that in turn is not induced to differentiate into the exocrine glandular phenotype (Acampora et al., 1996). 3. Early requirement of Otx2 for normal gastrulation and anterior neural plate induction and maintenance 3.1. Organisers and molecules in the current scenario of the anterior brain patterning Fate and patterning of tissues depend on the activity of organiser cells emanating signals to a responding tissue which undergoes morphogenetic changes resulting in a specific differentiated fate (Spemann and Mangold, 1924; Waddington, 1932; Gurdon, 1987). Indeed, in amphibians, the dorsal lip of the blastopore induces a new, ectopic secondary axis when transplanted on the ventral side of a host embryo. Because of this ability, the dorsal lip of the blastopore has been called the organiser (Spemann and Mangold, 1924). Further experiments in amphibian and chick embryos have suggested that the age of the organiser tissue influences the extension of the induced neural plate as well as its regional identity. An organiser deriving from an early gastrula induces anterior as well as posterior neural tissue, whereas a late organiser induces only posterior tissue (Gallera, 1971; Nieuwkoop et al., 1985; Storey et al., 1992). These results suggested the possibility that head and trunk inducing ability of the organiser might be associated to different cell populations coexisting in an early organiser. In mouse, at late streak stage the node is located at the rostral end of the primitive streak and is able to induce a secondary axis. Importantly, the secondary axis lacks any anterior neural tissues (Beddington, 1994) suggesting a functional parallelism with the amphibian late organiser. Inducing properties of an early mouse node have been tested in transplantation experiments, and also in this case it fails to induce anterior identity (Tam et al., 1997), thus indicating that, unlike the amphibian organiser, the mouse node is unable to induce rostral neuroectoderm, independently of its age. The mouse node gives rise to the ame that at mid-late streak stage underlies the anterior developing neuroectoderm in the midline, and comprises mesoderm (prechordal plate and notochord) and the definitive gut endoderm. These node-derived tissues are similar to those originated by the amphibian organiser and express similar genes (Beddington, 1981; Lawson et al., 1991). Moreover, there is clear evidence that the murine node and its derivatives are able both to emanate neuralising signals (Ruiz i Altaba, 1993, 1994; Beddington and Robertson, 1999) with patterning properties of different A/P value (Foley et al., 1997; Shimamura and Rubenstein, 1997) and to regulate the expression of the region-specific neural genes En1 and Otx2 in the neuroectoderm (Ang and Rossant, 1993; Ang et al., 1994). Interestingly, recent findings have ascribed to the AVE, which surrounds the epiblast cells at the pre-early streak stage, a crucial role in specifying anterior neural patterning in mouse (reviewed in Beddington and Robertson, 1998, 1999). Expression analysis and cell lineage studies remarkably contributed to define the origin and the molecular identity of the AVE. AVE precursor cells are located at the distal tip of the mouse pre-streak embryo and can be visualised by the expression of the Hex gene (Thomas et al., 1998). Few hours later, descendants of this group of cells will be found only in the perspective anterior region, giving rise to the first (molecular) asymmetry along the presumptive A/P axis of the embryo. This A/P asymmetry is confirmed by the analysis of the expression patterns of a number of genes such as Hex, Hesx1, goosecoid (gsc), cerberus-like (cer-l), Lim1, Otx2 and nodal (Simeone et al., 1993; Thomas and Beddington, 1996; Thomas et al., 1998; Belo et al., 1997; Varlet et al., 1997; Dattani et al., 1998). Cell ablation and tissue recombination experiments have indicated the functional relevance of AVE in inducing anterior patterning. Indeed, it has been shown that, (i) the removal of a patch of AVE cells expressing the Hesx1 gene prevents the subsequent expression of this gene in the rostral neuroectoderm which becomes D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 reduced and abnormally patterned (Thomas and Beddington, 1996); (ii) recombination of chick epiblast with rabbit pre-streak AVE induces the expression of forebrain markers, while chick hypoblast is unable to elicit the same response, thus suggesting that chick hypoblast and murine AVE might not share the property of specifying anterior neural patterning (Knötgen et al., 1999); (iii) chimera and transplantation experiments as well as the analysis of mouse mutants have indicated that a number of genes, including Lim1, Otx2 and nodal are required in the AVE for proper specification of the anterior neuroectoderm (Acampora et al., 1995; Shawlot and Behringer, 1995; Ang et al., 1996; Varlet et al., 1997), and in the ame for maintenance and refinement of correct identities (Acampora et al., 1998b; Rhinn et al., 1998; Shawlot et al., 1999); (iv) embryos homozygous for a null mutation in Cripto show expression, even if abnormal, of anterior neural markers in the absence of node-derived mesendoderm (Ding et al., 1998). This gene encodes a membrane-associated protein containing epidermal growth factor-like motifs and is expressed shortly before the onset of gastrulation in the proximal region of the epiblast where the primitive streak forms (Dono et al., 1993; Ding et al., 1998; Minchiotti et al., 2000). Cripto −/ − embryos lack a primitive streak and do not anteriorize the AVE, thus failing to convert the proximo-distal into A/P axis (Ding et al., 1998). Nevertheless, the AVE markers are correctly expressed, although in a distal position and the epiblast does express rostral neural markers such as Otx2 and En until 8 – 8.5 d.p.c., thus indicating that in the absence of a node and derived tissues the epiblast is able to acquire the identity of anterior neuroectoderm. Together with the ectopic transpantations of the node (Beddington, 1994; Tam et al., 1997), these results point to the possibility that in the mouse the AVE contains genetic information required to instruct the patterning of the rostral neuroectoderm and, hence, there might be two physically separated organising centres, AVE and node, responsible for the induction of head and trunk structures, respectively. This idea has been re-considered in the light of new mouse models recently generated. In particular, Chordin−/−; Noggin −/ − (Chd −/ − ; Nog − /−) double mutants have provided evidence that they are crucial in early forebrain development. These genes are expressed in the mouse node and its derivatives but not in the AVE, and single null mutation of either of them does not affect anterior neural patterning. However, Chd/Nog double mutants display severe defects in the development of prosencephalon (Bachiller et al., 2000). Analysis at the early stages of the mutant embryos has demonstrated that the AVE is correctly established, thus suggesting that either the ame cells have their own head-inducing properties which are affected in these mutants, or are required for the early maintenance of 75 anterior patterning initiated by the AVE, which per se might be necessary, but not sufficient, to induce the anterior neural plate. Early patterning of the CNS primordium is also controlled by additional mechanisms involving planar signals acting through the neuroectodermal plane (Doniach, 1993; Ruiz i Altaba, 1993, 1994). Furthermore, it has been shown that in zebrafish a small group of ectodermal cells located in the anteriormost head region is required for the patterning and survival of the anterior brain (Houart et al., 1998; Ruiz i Altaba, 1998). Finally, heterotopic transplantation studies have indicated that it is only from the synergistic interaction of anterior germinal layers (AVE and anterior epiblast) and a fragment of the posterior epiblast (early node) of early-streak embryos that it is possible to induce a full neural axis including anterior neural gene expression (Tam and Steiner, 1999). Similar experiments involving removal and ectopic transplantation of anterior midline tissue (AML, which includes both ame and ventral neuroectoderm) from late-streak embryos, have shown that AML is required for maintenance and regionalization of the forebrain (Camus et al., 2000). Among the genes required in the early specification of the anterior neural plate, Otx2 plays a remarkable role in both induction and maintenance of the rostral neural patterning (Simeone, 1998; Acampora and Simeone, 1999). These and other potential roles are now subject of intense study that takes advantage from genetically modified mouse models and embryological approaches. 3.2. Specification of anterior patterning requires Otx2 function In mouse, Otx2 is already transcribed before the onset of gastrulation in the epiblast and in the visceral endoderm (VE), and at the end of gastrulation in the ame and rostral neural plate (Simeone et al., 1992, 1993; Ang et al., 1994). During brain regionalization, Otx2 shows expression domains largely overlapping with those of Otx1, with a posterior border coincident with the mesencephalic side of the isthmic constriction (Simeone et al., 1992; Millet et al., 1996). Therefore, during gastrulation Otx2 is transcribed and translated in the cells that are believed to emanate signals in early specification and patterning of the neural plate (AVE and ame) as well as in those responding to these instructing signals (epiblast and anterior neuroectoderm) (reviewed in Simeone, 1998; Acampora and Simeone, 1999, Fig. 1A). The first indication that Otx2 is responsive to inductive interactions comes from explant-recombination experiments in gastrulating mouse embryos showing that a positive signal from ame of headfold stage embryos is able to maintain Otx2 expression in the anterior ectoderm of early 76 D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 Fig. 1. D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 streak embryos, and that a negative signal from the posterior mesendoderm, mimicked by exogenous retinoic acid (RA), represses Otx2 expression in the anterior ectoderm of late streak embryos (Ang et al., 1994). Similar interactions have been also demonstrated in Xenopus (Blitz and Cho, 1995). The possibility that RA might contribute to the early distinction between fore-midbrain and hindbrain by controlling Otx2 expression is supported by the finding that administration of exogenous RA at mid-late streak stage represses Otx2 expression in both the ame and the posterior neural plate (Ang et al., 1994; Simeone et al., 1995; Avantaggiato et al., 1996). This repression correlates with the appearance of microcephalic embryos that show early anteriorization of Hoxb1 expression, hindbrain expansion (Sive and Cheng, 1991; Conlon and Rossant, 1992; Marshall et al., 1992), loss of forebrain molecular and morphological landmarks, and gain of midbrain molecular markers in the rostralmost neuroectoderm (Simeone et al., 1995; Avantaggiato et al., 1996). Moreover, Otx2 responsiveness to RA application is a common feature in different species including Xenopus and chick (Bally-Cuif et al., 1995; Pannese et al., 1995). Nevertheless, the question of whether endogenous RA plays a physiological role in rostral CNS demarcation by contributing to the establishment of the posterior border of Otx2 expression, still remains open. The evidence that Otx2 may play a remarkable role in rostral CNS specification derives from in vivo genetic manipulation experiments performed in mouse and Xenopus which, to some extent, complement each other. In Xenopus, microinjection of synthetic Otx2 RNA results into an abnormal reduction in size of tail and trunk structures, and in the appearance of a second cement gland (Blitz and Cho, 1995; Pannese et al., 1995). These phenotypes have been interpreted either with a possible Otx2-mediated interference with move- 77 ments of extension and convergence during gastrulation (for trunk and tail reduction) and/or with an Otx2-requirement in the specification of anteriormost head structures (for the ectopic cement gland). Moreover, by using a dexamethasone-inducible OTX 2 protein it has been shown that the Xenopus Otx2 activity is regulated by regionally restricted factor(s), and that the cement gland-specific gene XCG may represent a direct target of the Otx2 gene product (Gammill and Sive, 1997). In mouse, Otx2 null embryos die early in embryogenesis, lack the rostral neuroectoderm fated to become forebrain, midbrain and rostral hindbrain, and show heavy abnormalities in their body plan (Fig. 1E) (Acampora et al., 1995; Matsuo et al., 1995; Ang et al., 1996). Heterozygous Otx2+ /− embryos into an appropriate genetic background show defects of the head such as serious brain abnormalities and craniofacial malformations, which are reminiscent of otocephalic phenotypes (Matsuo et al., 1995). The analysis of Otx2 null embryos revealed that at late streak stage, the rostral neuroectoderm is not specified and the primitive streak as well as the node and the ame are severely impaired. Therefore, one possibility is that the resulting headless phenotype might be due to the abnormal development of node-derived ame which lacks head organiser activity. A second possibility is that neural inducing properties of the AVE are severely impaired or abolished. In embryos replacing Otx2 with the lacZ reporter gene, the first abnormality is already detected at the early streak stage (Acampora et al., 1995). Indeed, at this stage, lacZ transcription and staining are abolished in the epiblast while remaining high in the VE of Otx2− /− embryos (Fig. 1D); the gsc expression is undetectable or confined to the proximal region of the mutant embryos (Acampora et al., 1995); and the presumptive AVE does not anteriorize, thus remaining confined to the distal region of the embryo (Fig. 1D). Fig. 1. Schematic representation and morphology of Otx2 − / − and hOtx12/hOtx12 mutant embryos as compared with wild type at different stages. In wild-type embryos at early streak stage (A) (6.5 d.p.c.) Otx2 mRNA and protein colocalize in VE and epiblast cells. Findings from Otx2 null embryos (D, E) suggest that in wild-type embryos (A–C) at the early-streak stage Otx2 is required in the VE to mediate signal(s) (arrows in A) that are directed to the epiblast and are required for specification of anterior patterning, while at late gastrula-headfold stage, Otx2 is required to maintain fore-midbrain regional identities (see also F – H) even though it cannot be assessed in which tissue (ame or neural plate) it plays this role. In null embryos (D, E), where Otx2 is replaced with the lacZ gene, the first impairment is seen at the pre-early streak stage (D) when lacZ transcription is lost in the epiblast and confined at the distal tip of the embryo. This observation indicates that at least one copy of the normal Otx2 allele is required in the VE to rescue signal(s) necessary for its transcription in the epiblast, for specification of anterior patterning and proper gastrulation. These findings suggest that Otx2 is an important component of VE organizing properties. The arrow in (E) points to the rostral limit of the neuroectoderm in an Otx2− /− embryo. In hOtx12/hOtx12 embryos (F – H), at early streak stage (F) (6.5 d.p.c.), hOtx1 transcripts are detected correctly in AVE and epiblast cells while, in contrast, the hOTX 1 protein is restricted to the VE. This model confirms the OTX 2 gene product requirement in the AVE for specification of the early anterior neural plate and demonstrates that hOTX 1 and OTX 2 proteins are functionally equivalent in the VE. Moreover, the differential post-transcriptional control of hOtx1 transcripts makes it possible to distinguish between specification and maintenance properties of Otx2. In fact, while the specification of the anterior neural plate and normal gastrulation are rescued by AVE-restricted hOTX 1 protein (F), the maintenance of anterior patterning is not recovered for the absence of any OTX protein in the epiblast-derived cells (anterior neural plate and ame) (G). This finding leads to the attractive hypothesis that Otx2-mediated maintenance properties (Otx2 translation in epiblast cells) might have been acquired during evolution to specify the vertebrate head. Abbreviations — AVE, anterior visceral endoderm; epi, epiblast; Hb, hindbrain; is, isthmus; Ms, mesencephalon; np, neural plate; Ov, otic vescicle; ps, primitive streak; Te, telencephalon; and VE, visceral endoderm. 78 D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 Therefore, these results indicate that headless phenotype and abnormal organisation of the primitive streak may be determined very early at the pre-early-streak stage by an impairment of AVE properties. Moreover, as revealed by the mesodermal early marker Brachyury (T), epiblast cells do not migrate posteriorly at the site of the primitive streak formation but remain for an abnormally longer period in a ring close to embryonic-extraembryonic boundary. Only later, and in a small number of Otx2 −/ − embryos, the presumptive AVE cells appear anteriorized. However, although abnormal, a primitive streak forms in all the Otx2 − /− embryos and mesodermal cells appear to be concentrated at the posterior third of the embryo (Acampora et al., 1995, 1998b; Ang et al., 1996). These findings, therefore, favour a relationship between primitive streak formation and anterior location of the AVE and suggest that Otx2, normally expressed in both epiblast cells and AVE, might be required in these two cell types in order to mediate proper positioning of the AVE and normal formation of the primitive streak. However, data deduced from the analysis of chimeric embryos and further mouse models indicate that early abnormalities in both AVE and primitive streak of Otx2 −/− embryos should be ascribed to Otx2 requirement in the VE (Acampora et al., 1998b; Rhinn et al., 1998; see below). Interestingly, an intriguing feature of Otx2 − /− embryos is that lack of anterior neuroectoderm is paralleled by failure of epiblast cells to express the lacZ reporter gene. Thus, since Otx2 is already transcribed from the earliest stages (unfertilised egg in Xenopus and at least morula in mouse), this observation suggests that maintenance of Otx2 transcription in the epiblast cells requires at least one normal allele expressed in the AVE while Otx2 transcription in the latter is independent of the presence of a normal allele (Simeone, 1998; Acampora and Simeone, 1999). These findings also support the existence of Otx2-mediated signal(s) emitted from the AVE and directed to the epiblast cells. Nevertheless, it is still unclear whether the same signal operates to mediate both specification of anterior patterning and Otx2 transcription in epiblast cells or these two events are independently controlled. 3.3. The role of Otx2 in the induction and maintenance of rostral CNS identities In order to understand the role of Otx2 in the specification of the anterior patterning, it is of particular relevance to define its functional contribution to the different tissues where it is expressed during gastrulation. A direct evidence proving a role for Otx2 in the AVE has been recently provided by generating murine chimeric embryos and new mouse models (Acampora et al., 1998b; Rhinn et al., 1998; Acampora et al., unpublished results). Chimeric embryos containing Otx2−/− epiblast and wild-type VE rescue an early Otx2−/− neural plate but subsequently fail to develop a brain, suggesting that Otx2 is firstly required in the AVE for induction of rostral neural plate and, then, in the epiblast-derived tissues for specification of forebrain and midbrain regional identities. Conversely, when chimeric embryos consist of an Otx2− /− VE and an Otx2+/+ epiblast, none of the phenotypic features of Otx2−/− embryos are rescued (Rhinn et al., 1998). This latter result also argues, as previously suggested by Otx2−/− mice (Acampora et al., 1995), that impaired ame of Otx2− /− embryos is a consequence of Otx2 requirement at earlier stages in the VE. Mice replacing Otx2 with Otx1 were originally generated in order to assess whether the two proteins shared functional equivalence or, alternatively, displayed unique properties specified by their limited amino acid divergence. Murine OTX 1 and OTX 2 gene products, in fact, share extensive sequence similarities even though in OTX1, downstream of the homeodomain, these regions of homology to OTX2 are separated by stretches of additional amino acids including repetitions of alanine and histidine residues (Simeone et al., 1993). Interestingly, homozygous mutant embryos replacing Otx2 with the human Otx1 (hOtx1) cDNA (hOtx12/ hOtx12) recover anterior neural plate induction and normal gastrulation but show a headless phenotype from 9 d.p.c. onwards (Fig. 1F –H). A combined analysis of both hOtx1 RNA and protein distribution during early gastrulation has revealed that while the hOtx1 mRNA is detected in the VE and epiblast, the hOTX1 protein is revealed only in VE (Fig. 1F). Nevertheless, this VE-restricted translation of the hOtx1 mRNA is sufficient to recover early anterior neural plate but fails to maintain fore-midbrain identities (Fig. 1G), and, consequently, hOtx12/hOtx12 embryos display a headless phenotype with a normal body plan (Fig. 1H) (Acampora et al., 1998b). In fact, at early-streak stage, hOtx12/hOtx12 embryos recover anteriorization of the AVE, normal primitive streak and proper expression of Lim1, cer-l, Hesx1, gsc and T. At late gastrula stage, the anterior patterning of the rostral neural plate is correctly defined by the expression of fore-, mid- and hindbrain markers such as Six3, Pax2, Gbx2 and Hoxb1 and the ame properly expresses Lim1, Noggin, cer-l and Hesx1. These findings support the idea, as indicated by chimeric studies (Rhinn et al., 1998) that Otx2 is required in the AVE for initiating the specification of the anterior patterning and demarcation of forebrain and midbrain territories (Acampora et al., 1998b). Further analysis of hOtx12/hOtx12 embryos reveals that at the early somite stage the forebrain markers BF1 and the hOtx12 mRNA are not detected in the rostral neuroectoderm where mid-hindbrain markers D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 such as Wnt1, En1, Fgf8, Gbx2 and Pax2 appear to be co-expressed. These observations lead to argue that the OTX2 gene product is required from the headfold stage onwards to maintain the anterior patterning previously established by the AVE. In this respect, the phenotype observed at the early somite stage appears to be the consequence of an A/P repatterning process involving the entire anterior neural plate (fore-midbrain) which, in the absence of any OTX gene product, adopts a more posterior fate (hindbrain) (Acampora et al., 1998b; Acampora and Simeone, 1999). Therefore, the hOtx12/hOtx12 mouse model allows to uncouple two distinct phases both requiring Otx2 early induction of anterior neural patterning that is under the control of AVE and its subsequent maintenance that is likely mediated by epiblast-derived cells (the ame and neuroectoderm). However, since Otx2 is normally transcribed and translated in both ame and rostral neuroectoderm, while the hOtx12 mRNA is transcribed but not translated either in the ame or in the rostral neuroectoderm, it cannot be deduced from this model whether Otx2 is required in one or both of these tissues to mediate maintenance of the anterior identity and whether hOtx1 is functionally equivalent to Otx2 also in these tissues. A cell-autonomous role of Otx2 in the neuroectoderm has emerged from the analysis of chimeras with a moderate contribution of Otx2 −/ − cells (Rhinn et al., 1999). It has been shown that genes such as Wnt1, Hesx1 and R-cadherin are selectively, not expressed in Otx2 − /− cells whereas other genes such as En2 and Six3 are uniformly expressed in neuroectodermal cells of both genotypes. How Otx2 is integrated in the network of other genetic functions which have been shown to be fundamental for anterior neural patterning is still an open question. The overall phenotype of Lim1 −/ − and hOtx12/hOtx12 embryos, for example, show impressive phenotypic similarities. Recently, the stage and the cell type in which Lim1 is required for head specification have been approached by chimera and tissue recombination experiments (Shawlot et al., 1999). These experiments have revealed that Lim1 is required in the AVE for inducing anterior neural patterning and, subsequently, in the ame to refine and maintain the anterior identity. Therefore, since maintenance of anterior pattern requires Otx2 in the ame or in the anterior neuroectoderm or in both tissues, it can be speculated that Lim1 might contribute to mediating the release of ame signal(s) instructing maintenance of anterior character and Otx2 might confer to neuroectoderm the competence to respond to this signal(s) emitted from the mesendoderm. This possibility is also compatible with a cell-autonomous role within the neuroectoderm and does not exclude an additional role also in the ame. 79 A recent in vitro study supports the possibility of a direct protein –protein interaction between OTX 2 Cterminus and Lim1 homeodomain (Nakano et al., 2000). 3.4. AVE-restricted OTX2 function is necessary for proper expression of Lim1 and bone morphogenetic protein (BMP) antagonists in the ame In hOtx12/hOtx12 (Acampora et al., 1998b) and chimera experiments (Rhinn et al., 1998), a tight correlation exists between correct specification of anterior patterning and the recovery of normal gastrulation. Moreover, in Otx2− /− embryos failure of anterior specification always coincides with a distal location of the AVE and abnormal gastrulation. In particular, in these embryos ame is no longer identifiable, and expression of Nog, Chd and Lim1 is strongly abnormal or absent (Acampora et al., 1998b; Rhinn et al., 1998). In hOtx12/hOtx12, general morphology as well as expression of these genes in the node and ame appears to be normal, and additionally, cer-l expression in the definitive endoderm emerging from the node also appears to be unaffected. As previously mentioned, recent studies have shown that (i) anterior midline tissue including ame and ventral neuroectoderm is required for maintenance and regionalization of forebrain (Camus et al., 2000); (ii) BMP antagonists such as Nog and Chd are required in a temporally coherent manner in the node and ame for forebrain development (Bachiller et al., 2000); and (iii) Lim1 is required in the ame for stabilising anterior patterning (Shawlot et al., 1999). On this basis, it can be hypothesised that anterior specification by AVE-restricted OTX function might act through ame-restricted non-cell autonomous properties of Chd, Nog and Lim1. This hypothesis does not exclude the existence of a direct inducing signal for anterior patterning emanating from the AVE. Rather it indicates that the VE is also important for normal development of the primitive streak (Beddington and Robertson, 1999). In this respect, it is noteworthy that chimera experiments performed to assess the role of HNF3b have indicated that this gene is necessary in the VE to promote proper primitive streak elongation (Dufort et al., 1998). Since, contrary to OTX2, hOTX1 protein is not detected in the ame, it cannot be excluded a priori that OTX2 also plays a role in these cells. Noteworthy is also the fact that in the absence of any OTX protein, hOtx12/hOtx12 embryos exhibited anterior patterning at least until 7.75 –8 d.p.c., while they subsequently fail in proper positioning of the IsO at the MHB. Chd −/ − ; Nog − /− embryos lacked anterior brain structures and retained a relatively normal midbrain (Bachiller et al., 2000). Together, these findings suggest that while early forebrain maintenance and/or induction is under 80 D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 the control of Chd/Nog signalling in the ame, OTX 2 is required for late maintenance by specifying midbrain territory and allowing the correct positioning of the IsO. 3.5. Specific and interchangeable roles between Otx1 and Otx2 Mutant phenotypes, expression patterns (see above) and amino acid sequence comparison support two possibilities, (i) the functional properties of Otx1 and Otx2 largely overlap and differences in their temporal and spatial transcriptional control are responsible for the highly divergent phenotypes of Otx1 −/ − and Otx2− /− mice; or (ii) OTX1 and OTX2 gene products display unique functional properties specified by their limited amino acid divergence. In order to distinguish between these two possibilities, mice models that replace Otx1 with the human Otx2 (hOtx2) cDNA and vice versa were generated. Homozygous mice in which Otx1 is replaced with the human Otx2 cDNA (hOtx21/hOtx21), despite a reduced expression of the transgenic alleles, no longer show epilepsy and corticogenic abnormalities caused by the absence of Otx1. This rescue is due to a restored normal cell proliferation activity in the dorsal neuroepithelium, as revealed by BrdU labelling experiments at 9.5 d.p.c. (Acampora et al., 1999a). This is particularly relevant when considering the different expression patterns of Otx1 and Otx2 genes in the dorsal telencephalon from the 9.5 d.p.c. stage onwards. Indeed, at this stage, while Otx1 is expressed throughout the entire dorsal telencephalon, Otx2 is expressed only in the mediodorsal area and basal neuroepithelium, whereas it disappears completely from the mediodorsal area by 11 d.p.c. Therefore, the rescue observed in hOtx21/hOtx21 mice suggests that Otx1 and Otx2 have interchangeable roles in the cortex. To complement the information derived by the loss-of-function and gene replacement experiments, it would be particularly interesting to see also the effects of an OTX over-dosage on the brain and, specifically, on cortical development. hOtx21/hOtx21 mice also show a significant improvement of mesencephalon, eye and lachrymal gland defects. Some of the Otx1 −/ − inner ear abnormalities are also rescued in the regions where the Otx genes are normally co-expressed, but not the absence of the lateral semicircular canal. As previously reported in detail, homozygous mutant mice in which Otx2 has been replaced with the human Otx1 (hOtx1) cDNA (hOtx12/ hOtx12) recover the anterior neural plate and proper gastrulation but fail to maintain fore-midbrain identities, displaying a headless phenotype from 9 d.p.c. onwards (Acampora et al., 1998b). A deeper analysis has revealed that despite RNA distribution in both the VE and epiblast, the hOTX1 protein was synthesised only in the VE, where it was sufficient to rescue VE-restricted Otx2 functions. In sum, these mouse models support an extended functional equivalence between OTX1 and OTX2 proteins and provide evidence that Otx1−/−; Otx2− /− contrasting phenotypes stem from differences in expression patterns rather than in amino acid sequences. The clearest exception to the overall Otx functional equivalence is provided by the lateral semicircular canal of the inner ear, that in hOtx21/hOtx21 mice is never restored (Morsli et al., 1999) as well as in mice in which Otx1 is replaced with the Drosophila otd gene (Acampora et al., 1998a). These findings, discussed below in evolutionary terms, suggest that the ability to specify the lateral semicircular canal of the inner ear may be, indeed, an Otx1-specific property (Acampora and Simeone, 1999). However, it is noteworthy that these studies do not address the question of whether hOTX1 might be functionally equivalent to OTX2 in the embryonic neuroectoderm and ame, due to the lack of hOTX1 protein in these tissues. Genetic replacement studies carried out by Suda et al. (1999) provide some evidence that OTX1 might be able to partially rescue the headless phenotype that was observed in hOtx12/hOtx12 mutant animals. However, it is unclear whether the amount of OTX1 was similar to that of OTX2 in these experiments (Suda et al., 1999). This is an important aspect since a reduction of OTX gene products below a critical threshold is always reflected in a mis-specification of fore- and midbrain regions (Acampora et al., 1997, 1998b; Suda et al., 1997; Broccoli et al., 1999; Millet et al., 1999; Simeone, 2000). In this context, it has been recently discovered that different roles attributed to two Hox genes belonging to the same paralogous group are the result of quantitative modulations in gene expression rather than of qualitative properties depending on protein sequence (Duboule, 2000; Greer et al., 2000). Thus, even if OTX1 and OTX2 do share a certain degree of functional equivalence in the neuroectoderm, the limited partial recovery of the phenotype might be ascribed either to a reduced level of OTX1 protein or to an OTX2-specific function. Further investigation is needed to address this important evolutionary aspect. 4. Brain patterning depends on a critical Otx gene dosage 4.1. Morphogenetic origin of the IsO The initial patterning of the primitive neuroepithelium is established during early gastrulation, when signals originating from both the underlying mesoderm and the VE or present within the ectoderm itself, D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 roughly divide the future CNS into few main subdivisions (Rubenstein and Shimamura, 1997; Beddington and Robertson, 1998). At the end of this process, different regions have acquired their own identity expressing a unique set of transcription factors. Later on, potent signalling centres are generated at the boundary between adjacent territories, which express diffusible molecules that refine and polarise the neighbouring neural tissue (Meinhardt, 1983; Rubenstein et al., 1998). The best studied centre is located at the MHB in the isthmic region. Over the last years, elegant tissue transplantation experiments in chick have addressed its role in neural patterning (Martinez et al., 1991, 1995; Marin and Puelles, 1994). In fact, when isthmic tissue is grafted to ectopic sites in the brain, as the caudal prosomeres or some rhombomeres, it can not only maintain its own identity, but can also induce the surrounding tissue to change its programmed fate giving rise to midbrain and cerebellar structures. Due to this potent non cell-autonomous function, the MHB signalling centre has been re-named IsO. However, within the forebrain, the territory rostral to the ZLI, the boundary between prosomeres 2 and 3, is not competent to respond to midbrain inducing signals released by the IsO (Martinez et al., 1991). In the last years, different proteins specifically expressed in the isthmic region and required for its development have been characterised. They include the transcription factors EN1, EN2, PAX2, PAX5 and two secreted molecules, WNT1 and FGF8 (Rowitch and McMahon, 1995; Joyner, 1996). Although some of these factors like EN2 and PAX5 appear to be general markers of the region, the dynamic expression profiles of the others (EN1, PAX2, WNT1 and FGF8) parallel the progressive refinement of specification taking place within the midbrain-hindbrain domain. In fact, if their expression domains are initially broad encompassing the presumptive midbrain and rostral hindbrain (in 1 – 5 somite old embryo), later on they become progressively restricted to narrow transverse rings that encircle the neural tube in the isthmic area (Bally-Cuif and Wassef, 1995). In particular, Wnt1 ring of expression is almost completely overlapped and localised at the caudal end of the prospective midbrain rostral-adjacent to the Fgf8 positive ring that lies on the isthmic-cerebellum anlage (Hidalgo-Sanchez et al., 1999b, Fig. 2). The functional role of all these genes (En, Pax, Fgf8 and Wnt1) has been tested in great detail in different animal models, clearly showing their requirement for the normal development of this region. In fact, mice homozygous for a Wnt1 null allele completely lack all the midbrain and isthmic derivatives (McMahon and Bradley, 1990; Thomas and Capecchi, 1990). Mutations in En1 cause a similar but milder phenotype (Wurst et al., 1994), whereas, mutations in En2 only lead to subtle defects in cerebellum cyto-organisation (Joyner et al., 1991). 81 However, En compound mutant mice lack the entire region resembling the Wnt1 mutant phenotype (W. Wurst and A.L. Joyner, unpublished results) and En2 can rescue the En1 mutant brain defects when it is expressed in place of En1, revealing overlapping functions between the two genes (Hanks et al., 1995). A similar brain deletion has been found also in mice carrying both Pax2 and Pax5 null alleles (Schwarz et al., 1997; Urbanek et al., 1997) and in the zebrafish noi mutants that harbour an induced mutation in the Pax2 orthologue (Brand et al., 1996; Lun and Brand, 1998). Likewise, Fgf8 mutant mice and zebrafish display an early brain deletion due to degeneration of the midbrain and isthmic tissue (Meyers et al., 1998; Reifers et al., 1998). In each mutant outlined so far, it has been reported that the expression of the other genes described is correctly initiated but no longer maintained. This is probably the cause that leads to the described loss of the brain structures (McMahon et al., 1992; Reifers et al., 1998; V. Blanquet and W. Wurst, unpublished results). These important findings strongly suggest a close functional connection among these genes, where the inactivation of a gene is able to feedback negatively on the transcription of all the other genes, leading to the degeneration of brain structures. The genetic maintenance loop among these genes is the molecular origin of the IsO and subsequent midbrain – hindbrain specification and morphological shaping (Fig. 3). This hypothesis is also supported by the striking phenotypes obtained in gain of function experiments. When, in fact, acrylic beads soaked with recombinant FGF8b protein are implanted in different areas of the caudal forebrain, the nearby regions are induced to change their fate into midbrain, cerebellar and isthmic structures (Crossley et al., 1996; Irving and Mason, 1999; Martinez et al., 1999). These results are mediated by the de-novo induction of Wnt1, Pax2, En2, En1 in the site of bead implantation. The same phenotype is obtained by inducing En gene expression ectopically in the caudal prosomeres either in zebrafish (Ristoratore et al., 1999) or chick (Shamim et al., 1999). Thus, single genes can trigger the activation of the entire genetic loop formed by Wnt, Fgf, Pax and En genes to initiate the neural fate re-specification. 4.2. Otx genes are required for correct positioning of the isthmus An important question to be answered is how all these genes are induced in this particular region of the developing neural tissue. Why not more anteriorly in the forebrain or more caudally in the spinal cord? Grafting or tissue ablation experiments in chick have shown that Fgf8 expressing tissue with properties of the IsO is generated when midbrain and rhombomere 1 tissue are juxtaposed but not when midbrain contacts 82 D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 Fig. 2. A schematic gene expression network in mice with different Otx2, Gbx2 or Fgf8 gene dosage that display a re-positioning of the MHB along the neural tube axis. In embryos with a decreasing Otx gene dosage (Otx1 −/ − ; Otx2 +/ − ), the Gbx2 (orange) and Fgf8 (grey) expression is abnormally spread into the rostral regions of the mesencephalon and 1st, 2nd, and 3rd prosomeres (p). The rostral shift of their expression domains cause a more anterior relocation of the MHB just near to the ZLI area. Moreover, the absence of OTX gene products in the neuroepithelium in hOtx12/hOtx12 mouse embryos cause the gene expression deregulation of Gbx2, Fgf8, and Wnt1 (violet) along all the neural plate. On the contrary, in gain of function experiments, the Otx2 ectopic expression in the metencephalon (met) leads to a repression of Fgf8 and Gbx2 activity in the same region, that positions the MHB more caudally (En1Otx2/ + ). In Gbx2 mutant embryos (Gbx2 −/ −), Otx2 and Wnt1 expression domains are enlarged caudally including rhombomere (rh) 3, and the mesencephalic tissue (mes) is expanded into the cerebellar anlage. Ectopic expression of Gbx2, under the control of the Wnt1 regulatory regions (Wnt1-Gbx2), leads to a transient expansion of the metencephalic region preceded by an ectopic rostral expression of Fgf8. The same results are obtained by ectopically expressing the Fgf8b spliced formed in the mesencephalon. Note that the nomenclature of the genotypes has not standardized and they are reported as cited in the original papers. D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 Fig. 3. Genetic hierarchy determining MHB formation. In the induction phase (7.5– 8.5 d.p.c.), Fgf8 expression is induced where the Otx2 and Gbx2 expression domains face each other. Recently, several reports have been shown that Fgf8 is activated when mesencephalic and metencephalic fated tissues are placed in contact. This secreted molecule is able to activate several transciption factors like PAX2, PAX5, EN1, EN2 and others that are necessary for the future specification and patterning of the region. All these molecules seem to maintain each other into an auto-regulatory loop. Moreover, FGF8 can re-induce Gbx2 expression, and inhibit Otx2 activity. any other rh or neural tissue (Hidalgo-Sanchez et al., 1999a; Irving and Mason, 1999). The genetic identity of the tissue rostral and adjacent to the Fgf8 expression domain is depending on Otx1 and Otx2 transcription factors (Simeone et al., 1993; Simeone, 1998). As previously mentioned, Otx2 −/ − embryos fail to specify forebrain, midbrain, and anterior hindbrain. The last region is specified by the IsO and never expresses Otx2 (Acampora et al. 1995; Matsuo et al., 1995; Ang et al., 1996). This finding argues in favour of an involvement of the Otx genes in the early IsO generation. Moreover, a more direct involvement of the Otx function in the anterior neuroepithelium specification is provided by the phenotype analysis of Otx compound mutants carrying only one Otx2 functional allele. In fact, while Otx1 −/− ; Otx2+/ − embryos do not display mesendoderm and gastrulation defects, they show molecular and morphological transformation of the caudal prosomeres 1 – 2 and mesencephalon into a strikingly enlarged metencephalon (Acampora et al., 1997). This brain re-patterning is the primary consequence of an abnormal enlargement of the Fgf8 expression do- 83 main towards the future diencephalic regions (Fig. 2) Therefore, a level above a critical threshold of Otx gene products is required to repress Fgf8 and, therefore, to maintain its correct transcript localisation at early somite stage. This molecular event triggers, few hours later, a rostral repositioning of En1 and Wnt1 expression domains followed by a more general anterior shift of the hindbrain specific markers and by failure of activation of the mesencephalic molecular determinants. Morphological alterations start to be scored at 10.5 d.p.c., when the isthmic region is repositioned in the caudal diencephalon, leading to replacement of the mesencephalic vesicle with a metencephalic-fated tissue (Acampora et al., 1997). Similar results are obtained when analysing the compound heterozygous embryos, Otx1+ /− ; Otx2+ /− in the CBA/C57 genetic background, where anterior expansion of rhombomere 1 combined with loss of mesencephalic tissue have been also described (Suda et al., 1997). These findings argue in favour of a negative feedback loop between Otx2 and Fgf8, that sharpens the two neighbouring boundaries of their complementary expression domains (Hidalgo-Sanchez et al., 1999b; Fig. 3). This hypothesis is strengthened by a different report (Martinez et al., 1999) that describes a strong repression of Otx2 expression in the chick mesencephalon around the place where a FGF8 secreting source is implanted. Moreover, the ectopic expression of the Fgf8b isoform under the control of the Wnt1 regulatory regions, inhibits the endogenous Otx2 expression in the mesencephalic anlage and tranforms this area in hindbrain-fated tissue (Liu et al., 1999; Fig. 2). An even stronger re-location of the IsO in the neuroepithelium is present in the homozygous hOtx12/hOtx12 embryos described previously (Acampora et al., 1998b). In this mouse model, where no OTX protein is present in epiblast derivatives, embryos normally undergo specification of the anterior neural plate which, however, fails to maintain its identity and acquires a more posterior fate, yielding a headless phenotype at late embryogenesis as assessed by the rostral mislocalisation at the rostral tip of the neuroectoderm of all the genes normally present in the IsO and rostral hindbrain, like Wnt1, Fgf8, Pax2, En1 and Gbx2, (Acampora et al., 1998b; Fig. 2). This finding provides a strong evidence for an Otx gene dosage requirement in anterior neural fate determination and following maintenance throughout a continued repression on the posteriorizing genetic determinants (Simeone, 1998). Is the action played by Otx genes only necessary or even sufficient to induce anterior fate in the neural plate? Gain of function experiments have been carried out, in the last years, to answer this question. As already mentioned, over-expression of Otx2 RNA in Xenopus results in an abnormal expansion of the head coupled with a strong reduction of the tail and trunk and with ectopic forma- 84 D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 tion of the most anterior structure of the Xenopus head, that is, the cement gland (Blitz and Cho, 1995; Pannese et al., 1995). To get a more specific and controlled Otx2 ectopic expression inside the neuroepithelium a knock-in approach has been devised for targeting the Otx2 coding region into the En1 genomic region (Broccoli et al., 1999). Therefore, the exogenous Otx2 allele becomes expressed ectopically in the rostral metencephalon where En1 expression domain is normally found, thus encompassing the isthmic region (Wassef and Joyner, 1997). The mice carrying this newly-engineered Otx2 allele (En1Otx2/ + ) display a striking alteration in the ratio between mesencephalic and cerebellar tissue. In fact, while the rectum is enlarged up to one-third, affecting in particular the inferior colliculi, the cerebellum loses almost completely its medial structure, called the vermis. Because of this brain rearrangement, the mice develop a strong ataxia during the early postnatal life, due to the compromised cerebellar functions (Broccoli et al., 1999). This malformation, already detectable in 10.5 d.p.c. embryos, is the final morphological outcome of a backward expansion of mesencephalic tissue at the expenses of the cerebellum. This repatterning process is driven by the knocked-in Otx2 allele that activates anteriorly expressed genes like En1, Wnt1 and EphrinA5 in its ectopic expression domain, whereas hindbrain molecular determinants such as Fgf8 and Gbx2 result repressed parallely. As a consequence, the IsO is shifted slightly caudally (Broccoli et al., 1999; Fig. 2). How far from its normal position can the IsO be shifted and up to what level of the A/P axis is neural tissue competent to respond to an Otx2 ectopic expression are the questions to be answered in the near future. While Otx2 seems to play a key role in determining the anterior fate of the neural plate, another homeobox gene, named Gbx2, has been individuated as the major molecular determinant in conferring the metencephalic identity (Bouillet et al. 1995; Chapman and Rathjen, 1995; von Bubnoff et al. 1995; Wassarmann et al., 1997). Gbx2 is expressed at very early stages of neuraxis development starting at 7.5 d.p.c., where it is expressed in all three germ layers of the gastrulating embryo in a region that extends rostrally from the posterior end of the embryo into the prospective hindbrain. Interestingly, its anterior expression boundary moves forward as the Otx2 expression domain retracts progressively into the perspective fore-midbrain territories (Conlon, 1995). This mutually excluding expression of these genes suggests a repression mechanism, either direct or indirect, between OTX 2 and GBX2 gene products. By 9.5 d.p.c., Gbx2 RNA is confined to a sharp transverse ring that is caudal immediately to the midbrain, and co-localises with Fgf8 and Pax2 expression domains. At this stage, Gbx2 expression is also detected in two longitudinal columns in the hindbrain and spinal cord (Bulfone et al., 1993; Wassarmann et al., 1997; Shamim and Mason, 1998; Hidalgo-Sanchez et al., 1999b). Its pivotal role in determining the rostral hindbrain neural identity has been assessed by gene targeting inactivation experiments (Wassarmann et al., 1997). In fact, Gbx2 null mutants die perinatally, lack the cerebellum, the locus coeruleus and the IV and V motor nuclei. These defects can be traced back to an early stage of neuroectoderm development (at least 8 d.p.c.) and are likely due to a failed specification of rhombomeres 1–3 and isthmic area that are replaced by a small undetermined region (Wassarmann et al., 1997; Fig. 2). Moreover, the midbrain is enlarged, extending caudally over its normal limit. This event is preceded by an abnormal caudal extension of the Otx2 expression domain, indicating Gbx2 as one of the factors that confines the Otx2 acitivity in the anterior neural plate. However, other unidentified factor(s) prevent Otx2 expression from expanding further caudally. To test the hypothesis that Gbx2 is involved in inhibiting Otx2 expression, Gbx2 was expressed in the midbrain at early somite stages under the control of the Wnt1 enhancer (Millet et al., 1999). Consistent with the initial assumption, the Otx2 caudal limit was shifted rostrally between the diencephalon and the mesencephalon, leading to an enlargement of the presumptive anterior hindbrain, and a rostral repositioning of the gene expression network that generates the IsO (Fgf8, Wnt1, En1 and Pax2; Fig. 2). Unfortunately, due to the Gbx2 transient ectopic expression, the transgenic embryos recover a normal proportion between the mesencephalon and the metencephalon by 12.5 d.p.c. (Millet et al., 1999). In conclusion, this large body of results strongly suggests that the reciprocal repression between Otx2 and Gbx2 is the first molecular event leading to the inductive process which will specify the midbrain and hindbrain (Fig. 3). In particular, this mutual repression is instrumental to three subsequent events occurring between 7.5 and 8.5 d.p.c. embryos, (i) a sharpening and positioning of the Otx2 and Gbx2 expression borders; (ii) the establishment of the mesencephalic and metencephalic identity, and (iii) the induction of the molecular cascade underlying the IsO genesis and its maintenance. Finally, the generation of conditional mouse mutants for Otx2 and Gbx2 as well as the isolation of their regulatory regions will shed more light in the near future on the mechanisms by which reasonably few transcription factors talk to each others to lay down the determination program leading to the final complex pattern of the CNS. D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 5. otd/Otx conserved functions throughout evolution 5.1. Otx genes in the animal kingdom Genes related to Drosophila otd and vertebrate Otx have been isolated from a wide range of organisms (Fig. 4). Most of them, up to protochordates have only one member, with few exceptions where duplication seems to have occurred in independent lineages (Li et al., 1996; Umesono et al., 1999). An Otx related gene is present already in Cnidarians, primitive metazoans with a defined body plan and radial symmetry. In these organisms, the Otx function is associated to cell movements involved in the formation of new axes rather than in the formation of the head (Smith et al., 1999). Rising in the evolutionary scale, Otx has been found in animals with primitive 85 bilateral symmetry such as planarians (Stornaiuolo et al., 1998; Umesono et al., 1999). In the planarian Dugesia tigrina, Otx expression has been found in regeneration blastemas after transverse sectioning, with an asymmetric pattern of transcripts more abundant in head regenerating tissues (Stornaiuolo et al., 1998). The expression of the Otx genes in these early metazoans reveals some features in common with chordate Otx genes. Although not directly correlated with a defined anterior structure, the ancient function seems to deal with patterning body axis and making tissues competent to respond to anteriorizing signals (Smith et al., 1999), at least in budding and regeneration processes which involve cell movements. Two Otx-related genes have been identified only on the basis of homeodomain sequence homology in the nematode C. elegans (Galliot et al., 1999). A third gene, more confidentially related Fig. 4. A simplified phylogenetic tree of the Metazoa indicating the major phyla and where Otx-related genes have been isolated. The asterisks points to the two possible positions of the first Otx duplication from a single ancestral gene. The presence of only one Otx-like gene in protochordates suggests that the Otx gene duplications observed in both Tribolium castaneum and in Dugesia japonica are likely independent duplication events occurred in these organisms. 86 D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 to Otx has been discovered by means of the sequencing project of the whole genome of this worm (Ruvkun and Hobert, 1998). However, no expression data are yet available about this gene. The first animal with a clearly head-associated Otx expression belongs to annelids (the leech Helobdella triserialis; Bruce and Shankland, 1998). This study is relevant particularly in evolutionary terms, since it supports the idea of the origin of bilaterians from radial ancestors (Brusca and Brusca, 1990). The passage from radials to bilaterians might have occurred through specification and subsequent expansion of a trunk precursor cell-population from one side of the radial ancestor. The leech Otx expression, which is organised radially around its mouth may represent a reminiscence of the Otx expression in a radial ancestor, thus suggesting that, if not recruited to specify trunk structures, relegation of head genes to head domain occurred in bilaterians as a consequence of their evolutionary origin. Otx expression in insects will be discussed in more detail in a separate section. The adult pentaradial symmetry shown by sea urchin seems to contradict the general head-associated Otx expression rule. It is held generally that the radial symmetry in echinoderms is a shared derived character (synapomorphy) because of their embryonic and larval bilateral symmetry (Lowe and Wray, 1997). Thus, the highly divergent and non-head specific Otx expression in sea urchin can be justified as a consequence of the highly modified body plan of this phylum. Comparative studies have demonstrated the existence of Otx-related genes in all chordates (Simeone et al., 1992, 1993; Frantz et al., 1994; Li et al., 1994; Mori et al., 1994; Bally-Cuif et al., 1995; Blitz and Cho, 1995; Mercier et al., 1995; Pannese et al., 1995; Kablar et al., 1996) including urochordates (Wada et al., 1996), cephalochordates (Williams and Holland, 1996), and agnathan vertebrates (Ueki et al., 1998), where they are expressed in the rostralmost CNS, independently of the complexity acquired by this area during evolution. The critical evolutionary position of lampreys will be discussed below, mainly with regard to Otx gene duplication. In urochordates and cephalochordates, only one Otx gene has been identified so far that may be related to Otx2 (Wada et al., 1996; Williams and Holland, 1998). Indeed, in addition to similarities in amino acid sequence and expression, they are both expressed during gastrulation in endoderm cells which suggests that their oldest and primary role might be to mediate signals required to specify anterior neuroectoderm. Restriction of an early widespread expression of Otx2-like genes to the anterior CNS is a remarkable feature of all vertebrates, which can be already observed in Ascidians and Amphioxus. This led to hypothesise the homology between fore-midbrain territory of vertebrates to the less- Fig. 5. Schematic comparison of expression domains of Otx-related genes (grey) during embryogenesis in some representative protochordates (Ascidia and Amphioxus) and vertebrates (Lamprey and mouse). Both lampreys Otx-related genes are shown because of their highly divergent expression patterns. Abbreviations — D, diencephalon; Ep, epiphysis; Ey, eye; F, forebrain; FE, frontal eye; HB, hindbrain; IO, infundibular organ; ll, lower lip; M, midbrain; MHB, mid-hindbrain boundary; NC, nerve cord; Oe, olfactory epithelium; Os, optic stalk; RV, rhomboencephalic vesicle; SC, spinal cord; SV, sensory vesicle; T, telencephalon; ul, upper lip; and VG, visceral ganglion. evoluted sensory vescicle and cerebral vescicle of Ascidians and Amphioxus, respectively (Fig. 5) (Williams and Holland, 1998). Some authors have also extended this homology further backwards in evolution. As mentioned previously, it has been proposed that a primitive Otx function could be associated only with cell movement rather than with anterior patterning (Smith et al., 1999). Similarly, functional data in frog (Blitz and Cho, 1995; Pannese et al., 1995) and mouse mutants (Acampora et al., 1995; Matsuo et al., 1995; Ang et al., 1996) suggest a possible involvement of Otx2 in controlling the cell movements occurring during gastrulation. Recently, an early role of the ascidian Otx2-related gene Hroth has been suggested in the inhibition of notochord and muscle cell fate or in the interference with notochord cell movements (Wada and Saiga, 1999). Conservation of the expression domains among Otx2-like orthologues from low chordates (Wada et al., 1996; Williams and Holland, 1996; Ueki et al., 1998), to vertebrates (Acampora and Simeone, 1999 and references therein) is consistent with the low rate of divergence of their alignable sequences. D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 The duplication event generating the Otx1 branch from the ancestor Otx2-like gene in gnathostome vertebrates cannot be dated precisely and will be discussed below. However, comparative sequence analysis indicates clearly that Otx1-like genes evolve more rapidly, as also shown by a further duplication event occurred in both Xenopus (Kablar et al., 1996) and Zebrafish (Mori et al., 1994) and by a ratio of sequence divergence higher than Otx2-like genes (Williams and Holland, 1998). These data can be reinforced by the profound changes in the expression domains of different vertebrate Otx1-like genes (Simeone et al., 1993; Mori et al., 1994) which underlie rapid evolution of regulatory sequences as well. 5.2. A common genetic program in insect and 6ertebrate head de6elopment Cloning of several master genes conserved throughout evolution and their comparative expression analysis has been used largely as a means to identify homologous body regions and molecular mechanisms among animals of different phyla (Abouheif et al., 1997). The most sensational example of such a functional conservation is represented by the Pax-6/eyeless gene, which in both Drosophila and vertebrates controls eye development (Callaerts et al., 1997). Until recently, it was assumed widely that the insect and vertebrate CNS had evolved independently (Garstang, 1928; Lacalli, 1994). This was due to their position on opposite body sides of the dorso-ventral (D/V) axis. One theory, the so-called ‘auricularia hypothesis’, postulated the homology between the outer ectoderm of the insect embryo and the chordate CNS, based on both anatomical studies made in echinoderms (auricularia larvae) and urochordates, and on comparative expression of the HOX genes. Starting from an ancient hypothesis of about two centuries ago postulated by Geoffroy Saint-Hilaire (De Robertis and Sasai, 1996), which has been object of controversial debate (Arendt and Nübler-Jung, 1994; Lacalli, 1995; Peterson, 1995), an increasing body of evidence has now accumulated which supports a common evolutionary origin of insect and vertebrate CNS. The first clues have been provided when it was shown that the overall arrangement of neuroblasts in three longitudinal columns on either side of the midline in both insect and vertebrate CNS (Doe and Goodman, 1985; Chitnis et al., 1995) was paralleled by conserved topographical expression (although with inverted D/V polarity) of pairs of homologous genes (NK-2/NK-2.2; ind/Gsh and Msh/Msx; Arendt and Nübler-Jung, 1996; D’Alessio and Frasch, 1996; Weiss et al., 1998). 87 Even more convincing was the similar expression of short gastrulation/chordin and decapentaplegic/Bmp4 pairs of homologous genes, which are antagonistic key molecules of the D/V patterning (Piccolo et al., 1997) in both Drosophila and vertebrates. As far as their expression is inverted with respect to the D/V axis in Drosophila and Xenopus, injection experiments have shown that these molecules are functionally equivalent (De Robertis and Sasai, 1996), thus supporting the existence of a homologous mechanism of D/V patterning in a common ancestor of both Drosophila and vertebrates and reinforcing the ancient hypothesis of an inversion of the D/V axis during evolution (De Robertis and Sasai, 1996; Arendt and Nübler-Jung, 1999). Finally, Gerhart (2000) has recently reviewed a number of hypotheses alternative to the inversion of the D/V axis, mainly based on the analysis of intermediate positions in evolution which imply intermediate anatomies, as in hemichordates. Along the A/P axis, in both Drosophila and vertebrates, the conserved families of HOM/HOX and otd/ Otx genes play a fundamental role in the regional specification of the neuroectoderm destined to form nerve cord/posterior brain and anterior brain, respectively. This gross similarity can be refined further when looking at the precise coincidence of gene-expression domains with the boundary of metameric units or neuromeres (Reichert and Simeone, 1999) and, as for the HOX genes, also according to the phenomenon of the ‘spatial colinearity’ (Lumsden and Krumlauf, 1996). Over the last 10 years, functional experiments have substanciated the equivalence suggested by the insect/ vertebrate comparative expression data. Most of these studies carried out in Drosophila have shown that mammalian HOX genes could either partially rescue phenotypes due to mutations of their fly orthologues or elicit responses similar to those elicited by their endogenous counterparts when transiently overexpressed (Malicki et al., 1990, 1993; Zhao et al., 1993; Bachiller et al., 1994). To further sustain the idea that some of the molecular mechanisms underlying brain development were conserved and comparable, a final, more challenging, proof remained to be verified. Could the Drosophila otd gene substitute for Otx genes in the mouse? That is, can a gene working in a structure as simple as the insect CNS substitute for homologous genetic functions in an enormously more complex organ such as the brain of mammals? The embryonic Drosophila brain is composed of two supraesophageal ganglia, each subdivided into three neuromeres. The anterior ganglion is subdivided into protocerebral, deutocerebral, and tritocerebral neuromeres. The gap gene otd is expressed mainly in the anteriormost (protocerebral) neuromere, which is deleted almost entirely in otd null embryos (Finkelstein and Perrimon, 1990; Cohen and Jürgens, 1991; Hirth et 88 D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 al., 1995; Younossi-Hartenstein et al., 1997). This phenotype is due to the failure of expression of the otd downstream gene lethal of scute, one of the proneural genes regulating the three-column arrangement of neuroblasts mentioned above. As a consequence, in the absence of otd, proneural genes are not activated and a gap-like deletion of the rostral brain neuromere (protocerebrum) results in late mutant embryos (Hirth et al., 1995). Other defects are also observed in the ventral nerve cord and in non-neural structures. Flies that are homozygotes for ocelliless (oc), a different otd allele, are viable and lack the ocelli (light sensing organs) and associated sensory bristles of the vertex (Finkelstein et al., 1990). Moreover, in cephalic development, different levels of OTD protein are required for the formation of specific subdomains of the adult head (Royet and Finkelstein, 1995). Despite the overall morphological differences, however, expression pattern and mutant phenotypes of Drosophila otd and mouse Otx genes can be paralleled (see previous sections) easily. Nevertheless, OTD and OTX proteins are highly conserved only in the homeodomain, which represents roughly onetenth of the whole OTD protein and about one-sixth and one-fifth of OTX 1 and OTX 2 proteins, respectively (Simeone et al., 1993). Outside the homeodomain, homology is restricted to a few very short sequences. Drosophila OTD protein also lacks the so-called ‘‘OTX tail’’ (Freud et al., 1997), a conserved motif of about 20 amino acids which is present in single copy in echinoderm, Ascidian and Amphioxus Otx-related genes, whilst is tandemly duplicated in all vertebrate OTX proteins at the COOH terminus (Williams and Holland, 1998). The limited sequence homology shared by OTD and OTX proteins underlines the importance that the homeodomain might have in triggering the CNS developmental programmes in both insects and vertebrates. Outside the homeodomain, the proteins could either have diverged, to allow mammals to acquire new and specific functions or might be more homologous in terms of tertiary structure than what the primary sequence alignment indicate. To gain insight into the possibility that otd and Otx genes might share conserved genetic functions during CNS development, we undertook experiments in which a Drosophila otd cDNA replaces both mouse Otx1 and Otx2 genes. When a full-coding Drosophila otd cDNA is introduced into a disrupted Otx1 locus by homologous recombination many abnormalities of the Otx1 − /− mice are rescued, regardless of a lower level of OTD (about 30%) as compared with the endogenous OTX 1 level (Acampora et al., 1998a). Homozygous knock-in otd mice (otd 1/otd 1) show no significant perinatal death (with respect to a 30% death of Otx1 −/ − newborns) and, most importantly, they have neither the abnormal behaviour nor EEG characteristics observed in the Otx1 null mutants. In otd 1/otd 1 adult mice, brain size as well as the thickness and cell number of the temporal and perirhinal cortices, both reduced in Otx1− /− mice, are very similar to wild-type. The rescue is likely to be ascribed at least in part, to a restored normal proliferating activity of the dorsal telencephalic neuroepithelium at 9.75 d.p.c. (Acampora et al., 1998a). As described in a previous section, Otx1 and Otx2 co-operate in brain morphogenesis and a minimal threshold (corresponding to either two copies of Otx2 or to one copy of Otx1 and one copy of Otx2) of their gene products is required for correct brain regionalization (Acampora et al., 1997). When otd is expressed in place of both copies of Otx1 and in the presence of one functional copy of Otx2 (otd 1/− ; Otx2+ /− or otd 1/otd 1; Otx2+/−), brain patterning abnormalities of the Otx1−/−; Otx2+ /− mutants are rescued partially in a otd dosedependent manner, both at morphological and molecular level (Acampora et al., 1998a). The extent of this rescue decreases progressively along the A/P axis, being the posterior mesencephalon still severely affected with respect to a normal telencephalon and to ameliorated diencephalic and anterior mesencephalic structures. All of these data indicate strongly that regionalization of the brain requires levels of OTX proteins that increase along the A/P axis and are particularly critical at the MHB (Acampora et al., 1999b). A partial rescue is also observed in some sensory and sensory-associated structures such as iris, ciliary process and Harderian glands. On the contrary, the lateral semicircular canal of the inner ear (last to be established in evolution) (Fritzsch et al., 1986; Torres and Giraldez, 1998) is never restored in otd 1/otd 1 mice, suggesting that, either it requires higher levels of protein or that specification of this structure is dependent upon an Otx1-newly established function. This seems indeed to be the case since, as previously mentioned, in hOtx21/hOtx21 mice, Otx2 is able to rescue some ear defects in the regions where both Otx genes are transcribed but not in the lateral semicircular canal, where only Otx1 is normally expressed (Acampora et al., 1999a; Morsli et al., 1999). The absence of the lateral canal in the inner ear of Otx1 − /− mice might represent a back-evolutionary mutation that can indicate the presumptive date of duplication of the Otx genes. This event should have occurred after that the lineage leading to cephalochordates had split from that leading to vertebrates (Williams and Holland, 1998) and probably after the latest passage leading from Agnatha to Gnathostomes. In fact, in lampreys, extant agnathan vertebrates, only two semicircular ducts (anterior and posterior) are present in the inner ear, and despite two Otx-like genes have been identified, none of them is clearly related to Otx1. However, it cannot be excluded that the Otx genes evolved by duplication in a common ancestor of D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 lampreys and gnathostomes (Fig. 4) and that the unclassified lamprey Otx represents a still evolutionary unstable version of an Otx1-like gene (Ueki et al., 1998). More recently, we have generated a mouse model in which it is the Otx2 gene to be substituted by the Drosophila otd cDNA (otd2), using the same targeting strategy as in the replacement with lacZ (Acampora et al., 1995) and with hOtx1 cDNA (Acampora et al., 1998b). Also in this case, the otd mRNA is detected in both AVE and epiblast, whereas the protein only in the VE. The OTD protein, exactly as the hOTX1 protein does, is able to take over all of the Otx2 functions in the AVE, thus recovering both gastrulation defects and absence of an early anterior neural plate due to the lack of Otx2. Later on, as in the hOtx12/hOtx12 mutants, however, otd 2/otd 2 embryos fail to maintain the anteriormost identities of the brain and become headless. These results, as far as limited to the AVE, provide a further proof of functional equivalence, shared by otd/ Otx genes, via the activation of the same basic genetic pathway(s). Similar conclusions have been drawn by complementary experiments in Drosophila (Leuzinger et al., 1998; Nagao et al., 1998). Heat-shock induced expression of hOTX1 and hOTX2 proteins in the fly is able to rescue the CNS defects of otd null mutant embryos (Leuzinger et al., 1998) as well as cephalic defects of the ocelliless mutations, both at the morphological and molecular level (Nagao et al., 1998), whereas in a wild-type background, OTX overexpression leads to induction of ectopic neural structures (Leuzinger et al., 1998). As previously mentioned, even though these crossphylum rescues highlight the fundamental role of the homeodomain because it is the only recognisable region conserved between OTD and OTX proteins, they do not exclude that functional equivalence may be extended to the overall structure of OTD/OTX proteins. The fact that OTD and OTX proteins are able to drive cephalic development through the activation of genetic pathways conserved between the two taxa, reinforces the idea that insect and chordate CNS are indeed homologous structures originated from a common ancestor and controlled by a common basic genetic program (Sharman and Brand, 1998; Acampora and Simeone, 1999; Reichert and Simeone, 1999). Interestingly, substitution of a different key gene involved in brain patterning processes with its Drosophila orthologue has led to very similar conclusions (Hanks et al., 1998). In fact, Drosophila engrailed was able to substitute for mouse Engrailed 1 (En1) functions in mid- and hind-brain regions but not in limb development. Therefore, despite a higher degree of homology between EN proteins with respect to OTD/ OTX proteins, this rescue reinforces the idea that some of the biochemical properties of highly conserved regu- 89 latory genes may be conserved across the two phyla and indicates that new functions have been acquired by the vertebrate genes during evolution. 5.3. Otx genes in brain e6olution One of the most interesting observations raised by our mouse models is the existence of a differential post-transcriptional control of the hOtx1/otd and Otx2 mRNAs between VE and epiblast cells. In heterozygous hOtx12/Otx 2 and otd 2/Otx 2 embryos, Otx2 mRNA and protein always colocalize, while the hOtx1 and otd mRNAs are translated only in the VE, thus suggesting that the knocked-in mRNAs detected in epiblast cells are post-transcriptionally regulated by an Otx2-independent cis-acting control (Acampora etal., 1998b). In Otx2+ /− embryos, the same Otx2 region that is replaced by the hOtx1 and otd cDNA is substituted with the lacZ gene (Acampora et al., 1995). In these embryos the lacZ mRNA is correctly detected in both AVE and epiblast while the b-gal staining is, again, heavily reduced in the epiblast at early-mid streak stage (Acampora et al., 1995). Therefore, three different mouse models replacing the same Otx2 genomic region with three different genes (lacZ, hOtx1 and otd) are suggestive of a different post-transcriptional control between AVE and epiblast cells. One or more Otx2 regions deleted in these models (introns, untranslated or coding sequences) should be responsible for this differential control. Loss of mRNA translation in the epiblast might be also influenced by abnormal molecular event(s) affecting RNA stability, processing and transport of the chimeric knocked-in transcripts. Whatever the impairments are, since in the AVE the mRNA is correctly translated, the absence of protein should be considered a peculiar event occurring in epiblast cells and their derivatives. The finding that Otx2 escapes this post-transcriptional control suggests that this is necessary for the maintenance of fore-midbrain territory specified by the AVE (Acampora et al., 1998b) and might have evolutionary implications. Indeed, the architectural components of the vertebrate brain (telencephalon, diencephalon and mesencephalon) are less clear in protochordates and a vertebrate-type brain, which is composed of a midbrain and six prosomers, firstly appears in Petromyzontoidea. It may be hypothesized that the specification of this prosomeric brain might have required the presence of a sufficient level of OTX2 protein in the early neuroectoderm cells and this event might have been acquired by modifying post-transcriptional control of Otx2 transcripts rather than its coding sequence which would have retained common functional properties among the otd-related genes through- 90 D. Acampora et al. / Progress in Neurobiology 64 (2001) 69–95 out evolution. The low ratio of Otx2 sequence divergence among the species fits with this hypothesis. Therefore, although this conservation in expression pattern and coding sequence might favour a remarkable role and functional equivalence of otd/Otx genes, it is unclear why the brain vescicles of protochordates have been so deeply and suddenly modified in a prosomeric territory that has been maintained in its basic topography until mammals (Rubenstein et al., 1998). A rather obvious answer to this question is that new genetic functions have been gained and recruited in developmental pathways. Indeed, it might be that conserved genes such as the Otx acquired different roles even while retaining an evolutionary functional equivalence. Based on this hypothesis, it is expected that drastic evolutionary events should act on the regulatory control (transcription and translation) of Otx-related genes rather than on their coding sequences. Interestingly, the findings that, (i) the Drosophila otd rescues in mouse most of the Otx1 −/ − impairments (Acampora et al., 1998a); (ii) the human Otx1 and Otx2 rescue most of the otd defects in flies (Leuzinger et al., 1998; Nagao et al., 1998; Sharman and Brand, 1998); (iii) Otx1 rescues Otx2 requirements in VE (Acampora et al., 1998b); (iv) Otx2 rescues most of the Otx1 − /− defects (Acampora et al., 1999a); (v) the Drosophila otd, similarly to Otx1, rescues Otx2 requirements in the VE (Acampora et al., unpublished results), indicate that Otx1, Otx2 and otd genes show a high degree of functional equivalence in the tissues and body regions where they are properly expressed. Therefore, these data support the notion that otd/Otx functions have been established in a common ancestor of fly and mouse and retained throughout evolution, while copy number and regulatory control of their expression have been modified and re-adapted by evolutionary events that have led to the specification of the increasingly complex vertebrate brain (Sharman and Brand, 1998; Simeone, 1998; Acampora and Simeone, 1999; Hirth and Reichert, 1999; Reichert and Simeone, 1999). Gene duplication may allow the duplicated gene to acquire new specific function(s) either retaining or losing ancestral properties, and similarly, modification of the regulatory control of gene expression may establish new expression patterns which might alter pre-existing cellfates by generating new specialised cellular functions. A likely consequence of both increased genomic complexity and modification of regulatory control of gene expression may result in an greater number of molecular interactions. This may contribute to modifying relevant morphogenetic processes that, in turn, can confer a change in shape and size of the body plan as well as in the generation of cell-types with new developmental potentials. On this basis, Otx gene duplication and subsequent or contemporary modification of regulatory control might have contributed to the evolution of the mammalian brain, for example by increasing the extent of neuroectodermal territory recruited to form the brain. This event might involve an improvement of proliferative activity of early neuronal progenitors (Acampora et al., 1998a, 1999a) and/or the positioning of the MHB (Acampora et al., 1997, 1998b; Suda et al., 1997). Additional property(ies) may be also conferred to the duplicated gene by altering its coding sequence. Thus, the limited amino acidic divergence between OTX1 and OTX2 might underlie modifications of their functional properties, as shown by the non-rescued absence of the lateral semicircular canal of the inner ear in mice replacing Otx1 with Otx2 (Acampora et al., 1996, 1999a; Morsli et al., 1999). 6. Conclusions In the last decade an impressive amount of knowledge has contributed to shed some light on the complexity of molecules and mechanisms involved in the development of the vertebrate brain. In this context otd/Otx genes play a cardinal role. Previous mouse models have indicated that Otx1 and Otx2 are required for normal brain and sense organ development and, together with the Drosophila orthodenticle (otd) gene they share a high degree of recriprocal functional equivalence. As far as the Otx genes are concerned, their interchangeability indicates that the differential transcriptional control between Otx1 and Otx2 is the major molecular reason responsible for generating Otx1 −/− and Otx2 − /− divergent phenotypes. Nevertheless, one of the most interesting observations raised by mouse models replacing Otx2 with hOtx1 or otd is the existence of a differential post-transcriptional and/or translational control between the VE and epiblast. Indeed, hOtx1 or otd mRNA were detected in VE, epiblast and its derivatives while hOTX1 or OTD proteins in the VE only. This event results in the failure of maintenance of fore-midbrain identities in the mutant embryos. In our opinion one of the most interesting perspectives will be the understanding of the molecular mechanism(s) underlying this phenomenon, and its potential relevance in the morphogenetic changes leading to the evolution of the mammalian brain. Acknowledgements We thank A. 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