Your search keyword '"Jonathan D.W. Clarke"' showing total 23 results

1. Coordinated assembly and release of adhesions builds apical junctional belts during de novo polarisation of an epithelial tube

Author

Jonathan D.W. Clarke, Andrew C. Symonds, Clare E. Buckley, and Charlotte A. Williams

Subjects

0303 health sciences, biology, Morphogenesis, Neural tube, biology.organism_classification, Transmembrane protein, Cell biology, 03 medical and health sciences, 0302 clinical medicine, Dual role, medicine.anatomical_structure, medicine, Solid organ, Molecular Biology, Zebrafish, RAB11A, 030217 neurology & neurosurgery, 030304 developmental biology, Developmental Biology, Lumen (unit)

Abstract

Using the zebrafish neural tube as a model, we uncover the in vivo mechanisms allowing the generation of two opposing apical epithelial surfaces within the centre of an initially unpolarised, solid organ. We show that Mpp5a and Rab11a play a dual role in coordinating the generation of ipsilateral junctional belts whilst simultaneously releasing contralateral adhesions across the centre of the tissue. We show that Mpp5a- and Rab11a-mediated resolution of cell-cell adhesions are both necessary for midline lumen opening and contribute to later maintenance of epithelial organisation. We propose that these roles for both Mpp5a and Rab11a operate through the transmembrane protein Crumbs. In light of a recent conflicting publication, we also clarify that the junction-remodelling role of Mpp5a is not specific to dividing cells.

Published

2020

2. Reversible Optogenetic Control of Subcellular Protein Localization in a Live Vertebrate Embryo

Author

Rachel E. Moore, Anna Reade, Orion D. Weiner, Jonathan D.W. Clarke, Anna R. Goldberg, Clare E. Buckley, Buckley, Clare [0000-0003-3329-3973], and Apollo - University of Cambridge Repository

Subjects

0301 basic medicine, Technology, Light, Biology, Optogenetics, Medical and Health Sciences, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, medicine, Animals, Molecular Biology, Zebrafish, phytochrome, Pard3, asymmetric inheritance, Neural tube, Embryo, Cell Biology, Biological Sciences, apico-basal polarity, biology.organism_classification, zebrafish, Protein subcellular localization prediction, 3. Good health, Transport protein, Cell biology, Multicellular organism, Protein Transport, 030104 developmental biology, medicine.anatomical_structure, Signal transduction, Developmental Biology, Signal Transduction

Abstract

Summary We demonstrate the utility of the phytochrome system to rapidly and reversibly recruit proteins to specific subcellular regions within specific cells in a living vertebrate embryo. Light-induced heterodimerization using the phytochrome system has previously been used as a powerful tool to dissect signaling pathways for single cells in culture but has not previously been used to reversibly manipulate the precise subcellular location of proteins in multicellular organisms. Here we report the experimental conditions necessary to use this system to manipulate proteins in vivo. As proof of principle, we demonstrate that we can manipulate the localization of the apical polarity protein Pard3 with high temporal and spatial precision in both the neural tube and the embryo’s enveloping layer epithelium. Our optimizations of optogenetic component expression and chromophore purification and delivery should significantly lower the barrier for establishing this powerful optogenetic system in other multicellular organisms., Graphical Abstract, Highlights • The phytochrome system has been optimized for use within multicellular organisms • Protein recruitment can be tightly controlled to a specific subcellular region • Protein recruitment occurs with high binding and reversal kinetics • The subcellular localization of the apical polarity protein Pard3 is manipulated, The phytochrome system is a powerful tool that is used to manipulate protein localization. Here, Buckley et al. optimize the phytochrome system in live zebrafish embryos and demonstrate rapid and reversible protein recruitment to specific subcellular regions within specific cells, at a high spatial and temporal resolution.

Published

2016

3. Requirement for the zebrafish mid-hindbrain boundary in midbrain polarisation, mapping and confinement of the retinotectal projection*

Author

Michael Brand, Jonathan D.W. Clarke, Frank Reifers, Caroline H. Brennan, Alexander Picker, and Nigel Holder

Subjects

animal structures, Fibroblast Growth Factor 8, Genotype, Hindbrain, Biology, Ligands, Midbrain, FGF8, medicine, Animals, RNA, Messenger, TECTA, Molecular Biology, In Situ Hybridization, Zebrafish, Genetics, Brain, Ephrin-A2, Gene Expression Regulation, Developmental, Membrane Proteins, Ephrin-A5, Immunohistochemistry, Cell biology, Fibroblast Growth Factors, Phenotype, medicine.anatomical_structure, nervous system, Retinal ganglion cell, Mutation, Tissue Transplantation, embryonic structures, Ephrin A5, sense organs, Ephrin A2, Tectum, Transcription Factors, Developmental Biology

Abstract

The organizer at the midbrain-hindbrain boundary (MHB organizer) has been proposed to induce and polarize the midbrain during development. We investigate the requirement for the MHB organizer in acerebellar mutants, which lack a MHB and cerebellum, but retain a tectum, and are mutant for fgf8, a candidate inducer and polarizer. We examine the retinotectal projection in the mutants to assay polarity in the tectum. In mutant tecta, retinal ganglion cell (RGC) axons form overlapping termination fields, especially in the ventral tectum, and along both the anterior-posterior and dorsal-ventral axis of the tectum, consistent with a MHB requirement in generating midbrain polarity. However, polarity is not completely lost in the mutant tecta, in spite of the absence of the MHB. Moreover, graded expression of the ephrin family ligand Ephrin-A5b is eliminated, whereas Ephrin-A2 and Ephrin-A5a expression is leveled in acerebellar mutant tecta, showing that ephrins are differentially affected by the absence of the MHB. Some RGC axons overshoot beyond the mutant tectum, suggesting that the MHB also serves a barrier function for axonal growth. By transplanting whole eye primordia, we show that mapping defects and overshooting largely, but not exclusively, depend on tectal, but not retinal genotype, and thus demonstrate an independent function for Fgf8 in retinal development. The MHB organizer, possibly via Fgf8 itself, is thus required for midbrain polarisation and for restricting axonal growth, but other cell populations may also influence midbrain polarity.

Published

1999

4. Selective expression of purinoceptor cP2Y1 suggests a role for nucleotide signalling in development of the chick embryo

Author

Ketan Patel, Andrea Townsend-Nicholson, Jonathan D.W. Clarke, Geoffrey Burnstock, and Martin P. Meyer

Subjects

Central Nervous System, P2Y receptor, Time Factors, Limb Buds, Chick Embryo, Biology, Receptors, Purinergic P2Y1, Extracellular, Animals, Tissue Distribution, In Situ Hybridization, Receptors, Purinergic P2, Mesonephros, fungi, Embryogenesis, Purinergic receptor, Receptors, Purinergic, Gene Expression Regulation, Developmental, Embryo, Blotting, Northern, Embryonic stem cell, Molecular biology, Branchial Region, Somites, embryonic structures, Developmental biology, Developmental Biology

Abstract

Responses to extracellular nucleotides (e.g., ATP, ADP, etc.) have been demonstrated in a number of embryonic cell types suggesting they may be important signalling molecules during embryonic development. Here the authors describe for the first time the expression of a G-protein–coupled receptor for extracellular ATP, chick P2Y1 (cP2Y1), during embryonic development of the chick. During the first 10 days of embryonic development, cP2Y1 is expressed in a developmentally regulated manner in the limb buds, mesonephros, brain, somites, and facial primordia, suggesting that this receptor may have a role in the development of each of these systems. Dev Dyn 1999;214:152–158. © 1999 Wiley-Liss, Inc.

Published

1999

5. Stability and Plasticity of Neural Crest Patterning and Branchial Arch Hox Code after Extensive Cephalic Crest Rotation

Author

Paul Hunt, Paul Buxton, Jonathan D.W. Clarke, Peter Thorogood, and Patrizia Ferretti

Subjects

animal structures, Ectomesenchyme, Branchial arch, Chick Embryo, Biology, Mesoderm, 03 medical and health sciences, 0302 clinical medicine, Cell Movement, Morphogenesis, Animals, Maxillofacial Development, 10. No inequality, Hox gene, Molecular Biology, Fluorescent Dyes, 030304 developmental biology, Homeodomain Proteins, 0303 health sciences, Histocytochemistry, Gene Expression Regulation, Developmental, Neural crest, Cell Biology, Anatomy, Neural Crest, Tissue Transplantation, embryonic structures, Crest, Neural crest cell migration, Branchial Region, Neural plate, 030217 neurology & neurosurgery, Developmental Biology

Abstract

The extent to which the spatial organisation of craniofacial development is due to intrinsic properties of the neural crest is at present unclear. There is some experimental evidence supporting the concept of a prepattern established within crest while contiguous with the neural plate. In experiments in which the neural tube and premigratory crest are relocated within the branchial region, crest cells retain patterns of gene expression appropriate for their position of origin after migration into the branchial arches, resulting in skeletal abnormalities. But in apparent conflict with these findings, when crest is rerouted by late deletion of adjacent crest, infilling crest alters its pattern of gene expression to match its new location, and a normal facial skeleton results. In order to reconcile these findings and thus identify processes of relevance to the course of normal development, we have performed a series of neural tube and crest rotations producing a more extensive reorganisation of cephalic crest than has been previously described. Lineage analysis using DiI labelling of crest derived from the rotated hindbrain reveals that crest does not migrate into the branchial arch it would have colonised in normal development, rather it simply populates the nearest available branchial arches. We also find that crest adjacent to the grafted region contributes to a greater number of branchial arches than it would in normal development, resulting in branchial arches containing mixed cell populations not occurring in normal development. We find that after exchange of first and third arch crest by rotation of r1–7, crest alters its expression ofhoxa-2andhoxa-3to match its new location within the embryo resulting in the reestablishment of the normal branchial arch Hox code. A facial skeleton in which all the normal components are present, with some additional ectopic first arch structures, is formed in this situation. In contrast, when second and third arch crest are exchanged by rotation of r3 to 7, ectopic Hox gene expression is stable, resulting in the persistence of an abnormal branchial arch Hox code and extensive defects in the hyoid skeleton. We suggest that the intrinsic properties of crest have an effect on the spatial organisation of structures derived from the branchial arches, but that exposure to increasingly novel environments within the branchial region or “community effects” within mixed populations of cells can result in alterations to crest Hox code and morphogenetic fate. In both classes of operation we find that there is a tight link between the resulting branchial arch Hox code and a particular skeletal morphology.

Published

1998

6. Mirror-symmetric microtubule assembly and cell interactions drive lumen formation in the zebrafish neural rod

Author

Claudio Araya, Brian A. Link, Xiaoyun Ren, Brian S. Clark, Clare E. Buckley, Jonathan D.W. Clarke, Mary J. Green, Gemma C. Girdler, Laura C. Ward, Buckley, Clare [0000-0003-3329-3973], and Apollo - University of Cambridge Repository

Subjects

Neural Tube, Embryo, Nonmammalian, Cell division, Recombinant Fusion Proteins, Green Fluorescent Proteins, Lumen (anatomy), Cell Communication, Biology, Microtubules, Article, General Biochemistry, Genetics and Molecular Biology, chemistry.chemical_compound, Microtubule, Cell Movement, Cell polarity, medicine, Animals, Molecular Biology, Zebrafish, Neurulation, Body Patterning, Luminescent Agents, General Immunology and Microbiology, General Neuroscience, Nocodazole, Neural tube, Cell Polarity, Zebrafish Proteins, biology.organism_classification, Tubulin Modulators, Cell biology, Protein Transport, medicine.anatomical_structure, chemistry, rab GTP-Binding Proteins, Mutation, Carrier Proteins, Cell Division

Abstract

By analysing the cellular and subcellular events that occur in the centre of the developing zebrafish neural rod, we have uncovered a novel mechanism of cell polarisation during lumen formation. Cells from each side of the neural rod interdigitate across the tissue midline. This is necessary for localisation of apical junctional proteins to the region where cells intersect the tissue midline. Cells assemble a mirror-symmetric microtubule cytoskeleton around the tissue midline, which is necessary for the trafficking of proteins required for normal lumen formation, such as partitioning defective 3 and Rab11a to this point. This occurs in advance and is independent of the midline cell division that has been shown to have a powerful role in lumen organisation. To our knowledge, this is the first example of the initiation of apical polarisation part way along the length of a cell, rather than at a cell extremity. Although the midline division is not necessary for apical polarisation, it confers a morphogenetic advantage by efficiently eliminating cellular processes that would otherwise bridge the developing lumen.

Published

2013

7. Late effects of retinoic acid on neural crest and aspects of rhombomere

Author

Malcolm Maden, Victoria E. Prince, Andrew Lumsden, Nigel Holder, Emily Gale, and Jonathan D.W. Clarke

Subjects

Cell type, Molecular Sequence Data, Retinoic acid, Rhombomere, Tretinoin, Hindbrain, Chick Embryo, Biology, chemistry.chemical_compound, Cell Movement, Morphogenesis, medicine, Animals, RNA, Messenger, Molecular Biology, Early Growth Response Protein 2, DNA Primers, Homeodomain Proteins, Base Sequence, Genes, Homeobox, Gene Expression Regulation, Developmental, Neural crest, Anatomy, Motor neuron, Cell biology, DNA-Binding Proteins, Rhombencephalon, Phenotype, medicine.anatomical_structure, chemistry, Neural Crest, Trans-Activators, Ectopic expression, Crest, Transcription Factors, Developmental Biology

Abstract

We exposed st.10 chicks to retinoic acid (RA), both globally, and locally to individual rhombomeres, to look at its role in specification of various aspects of hindbrain derived morphology. Previous studies have looked at RA exposure at earlier stages, during axial specification. Stage 10 is the time of morphological segmentation of the hindbrain and is just prior to neural crest migration. Rhombomere 4 localised RA injections result in specific alterations of pathways some crest cells that normally migrate to sites of differentiation of neurogenic derivatives. The r4 crest cells that give rise to mesenchymal derivatives are unaffected. In addition, r4 gene expression is also partially altered by RA; within 6 hours of r4 exposure to RA, ectopic expression of Krox-20 is seen in r4 and Hoxb-1 expression is lost while Hoxa-2 expression continues normally. When we examined these RA-treated animals later in development, they showed an anterior displacement of the facial ganglion in addition to a mis-direction of the extensions of its distal axons and a dramatic decrease in the number of contralateral vestibuloacoustic neurons normally seen in r4. Only this r4-specific neuronal type is affected in r4; the motor neuron projections seem normal in experimental animals. The specificity of this result, combined with the loss of Hoxb-1 expression in r4 and the work by Krumlauf and co-workers showing gain of contralateral neurons co-localised with ectopic Hoxb-1 expression, indicates a role for Hoxb-1 and RA in the specification of this cell type in normal development. These results suggest that RA, at st.10, is able to affect some aspects of segment identity while leaving others unchanged.

Published

1996

8. Ectopic expression of Hoxa-1 in the zebrafish alters the fate of the mandibular arch neural crest and phenocopies a retinoic acid-induced phenotype

Author

E. Oxtoby, T. Jowett, Jonathan D.W. Clarke, Yi-Lin Yan, D. Alexandre, and Nigel Holder

Subjects

Molecular Sequence Data, Rhombomere, Retinoic acid, Tretinoin, Hindbrain, Mandible, chemistry.chemical_compound, medicine, Animals, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Hox gene, Molecular Biology, Zebrafish, Homeodomain Proteins, Base Sequence, Sequence Homology, Amino Acid, biology, Genes, Homeobox, Gene Expression Regulation, Developmental, Neural crest, biology.organism_classification, Molecular biology, Rhombencephalon, Phenotype, chemistry, Neural Crest, embryonic structures, Trans-Activators, Ectopic expression, Sequence Alignment, Developmental Biology, medicine.drug

Abstract

Considerable evidence has demonstrated that retinoic acid influences the formation of the primary body axis in vertebrates and that this may occur through the regulation of Hox gene expression. In this study, we show that the phenotype induced by exogenous retinoic acid in the zebrafish can also be generated by the overexpression of Hoxa-1 following injection of synthetic RNA into the fertilised egg. The isolation, sequence and expression pattern of the zebrafish Hoxa-1 gene is described. We show that exogenously applied retinoic acid causes the ectopic accumulation of Hoxa-1 message during gastrulation in the hypoblast in the head region. Overexpression of Hoxa-1 following injection of RNA causes abnormal growth of the anterior hindbrain, duplication of Mauthner neurons in rhombomere (r) 2 and fate changes of r2 mesenchymal and neurogenic neural crest. These results are discussed in terms of the role of Hoxa-1 in controlling anterior hindbrain patterning and the relationship between expression of Hoxa-1 and retinoic acid.

Published

1996

9. Early phenotypic choices by neuronal precursors, revealed by clonal analysis of the chick embryo hindbrain

Author

Scott E. Fraser, Roger J. Keynes, Andrew Lumsden, and Jonathan D.W. Clarke

Subjects

Neurons, Stem Cells, Neurogenesis, Central nervous system, Rhombomere, Cell Differentiation, Hindbrain, Embryo, Chick Embryo, Anatomy, Biology, Phenotype, Clone Cells, Cell biology, Rhombencephalon, medicine.anatomical_structure, Microscopy, Fluorescence, nervous system, Precursor cell, medicine, Animals, Molecular Biology, Mitosis, Developmental Biology

Abstract

The mechanisms that generate diverse neuronal phenotypes within the central nervous system are thought to involve local cues or cell-cell interactions acting late in neurogenesis, perhaps as late as the last precursor cell division. We describe here a clonal analysis of neuronal development in the chick hindbrain, using an intracellular tracer to mark single precursor cells, that suggests the operation of an alternative strategy. The majority of clones, ranging from 1 to 46 cells, contained neurons of only one of several possible phenotypes. These single-phenotype clones were not positionally restricted within a rhombomere but were interspersed with other clones containing distinct phenotypes. The assignment of neuronal phenotype in this brain region may, therefore, be made in early precursors and remembered through several rounds of mitotic expansion and dispersal.

Published

1994

10. Segmental repetition of neuronal phenotype sets in the chick embryo hindbrain

Author

Jonathan D.W. Clarke and Andrew Lumsden

Subjects

Cell type, Central nervous system, Rhombomere, Hindbrain, Chick Embryo, Biology, Neural Pathways, medicine, Animals, Molecular Biology, Horseradish Peroxidase, Neurons, Histocytochemistry, Embryogenesis, Embryo, Anatomy, Phenotype, Axons, Rhombencephalon, medicine.anatomical_structure, Microscopy, Fluorescence, nervous system, Neuron, Neuroscience, Developmental Biology

Abstract

The neurons within the segmented hindbrain of the early chick embryo have been mapped with the neuronal tracers HRP and fluorescent lysinated dextran. We have categorised neurons according to their axonal pathways and have then compared rhombomeres with respect to the number and class of neurons present. The results indicate that most rhombomeres are similar in that they contain the same set of basic neuronal types but differ in that particular neuronal types are more abundant in some rhombomeres than others. The data support the concept that the hindbrain develops according to ‘variations on a segmental theme’ rather than ‘each segment is unique’. Many of the cell types occupy distinct mediolateral domains that are probably established by both the differential migration of some neuronal classes and the spatial segregation of distinct precursors. The caudal rhombomeres 7 and 8 are exceptional in that they do not have the full set of basic neuronal types and also contain two additional medial cell types that are not present rostrally. The mechanisms that may generate the regional diversity apparent in the more mature hindbrain are discussed.

Published

1993

11. Focal Electroporation in Zebrafish Embryos and Larvae

Author

Isaac H. Bianco, Jonathan D.W. Clarke, and Marcel Tawk

Subjects

Gene knockdown, animal structures, Morpholino, Electroporation, Embryo, Biology, biology.organism_classification, Molecular biology, Cell biology, Fate mapping, embryonic structures, Ectopic expression, Developmental biology, Zebrafish

Abstract

A method is described that allows the introduction by electroporation of either small dyes or larger RNA, DNA, or morpholino constructs into single cells or small groups of cells in zebrafish embryos or larvae. The dye or construct is delivered to cells via a patch-like microelectrode that also delivers the electroporation stimulus train. This technique allows the experimenter to target cells of their choice at a particular time of development and at a particular location in the embryo, and is useful for fate mapping, analysing neuronal organisation, ectopic expression and gene knockdown experiments.

Published

2009

12. Using Fluorescent Dyes for Fate Mapping, Lineage Analysis, and Axon Tracing in the Chick Embryo

Author

Jonathan D.W. Clarke

Subjects

Axon tracing, Lineage (genetic), Fate mapping, Embryo, Biology, Molecular biology, Cell biology

Published

2008

13. Hedgehog signalling maintains the optic stalk-retinal interface through the regulation of Vax gene activity

Author

Stephen W. Wilson, Jonathan D.W. Clarke, and Masaya Take-uchi

Subjects

medicine.medical_specialty, Nodal Protein, Recombinant Fusion Proteins, Nodal signaling, Receptors, Cell Surface, Biology, Xenopus Proteins, Retina, Receptors, G-Protein-Coupled, Transforming Growth Factor beta, Internal medicine, medicine, Animals, Humans, Optic stalk, Hedgehog Proteins, Sonic hedgehog, Eye Proteins, Molecular Biology, In Situ Hybridization, Phylogeny, Zebrafish, Body Patterning, Homeodomain Proteins, Neuropeptides, Genes, Homeobox, Gene Expression Regulation, Developmental, Optic Nerve, Optic vesicle, Zebrafish Proteins, Receptors, Fibroblast Growth Factor, Smoothened Receptor, Cell biology, Coloboma, medicine.anatomical_structure, Endocrinology, Gene Expression Regulation, Optic nerve, biology.protein, Trans-Activators, sense organs, Smoothened, Developmental Biology, Signal Transduction

Abstract

During early formation of the eye, the optic vesicle becomes partitioned into a proximal domain that forms the optic nerve and a distal domain that forms the retina. In this study, we investigate the activity of Nodal,Hedgehog (Hh) and Fgf signals and Vax family homeodomain proteins in this patterning event. We show that zebrafish vax1 and vax2 are expressed in overlapping domains encompassing the ventral retina, optic stalks and preoptic area. Abrogation of Vax1 and Vax2 activity leads to a failure to close the choroid fissure and progressive expansion of retinal tissue into the optic nerve, finally resulting in a fusion of retinal neurons and pigment epithelium with forebrain tissue.We show that Hh signals acting through Smoothened act downstream of the Nodal pathway to promote Vax gene expression. However, in the absence of both Nodal and Hh signals, Vax genes are expressed revealing that other signals,which we show include Fgfs, contribute to Vax gene regulation. Finally, we show that Pax2.1 and Vax1/Vax2 are likely to act in parallel downstream of Hh activity and that the bel locus (yet to be cloned) mediates the ability of Hh-, and perhaps Fgf-, signals to induce Vax expression in the preoptic area. Taking all these results together, we present a model of the partitioning of the optic vesicle along its proximo-distal axis.

Published

2003

14. A reciprocal relationship between cutaneous nerves and repairing skin wounds in the developing chick embryo

Author

Jonathan D.W. Clarke, Steven Harsum, and Paul Martin

Subjects

animal structures, Time Factors, sensory nerves, Ultraviolet Rays, embryo, Stimulation, Hindlimb, Chick Embryo, Biology, Animals, Process (anatomy), Molecular Biology, hyperinnervation, Skin, Skin repair, Inflammation, Neurons, Wound Healing, integumentary system, Neural crest, Embryo, Anatomy, Cell Biology, chick, Neural Crest, Microscopy, Electron, Scanning, Cutaneous innervation, Wound healing, Developmental Biology

Abstract

Various studies have suggested that the rate of adult skin healing may be in some way dependent on signals emanating from cutaneous nerves. Further, it appears that adult wounds become hyperinnervated by sensory nerves during the process of healing. In order to investigate this reciprocal relationship further, we have used a simple embryonic model to look at the effect of wounds on nerves, and conversely, the effect of nerves on wounds. We find that wounds made to the dorsum of the chick wing bud, at a stage prior to normal innervation (at E4), or soon after the normal establishment of cutaneous innervation (at E7), subtly alter the pattern of branching by perturbing developmental guidance cues, but do not cause hyperinnervation, whereas wounding at E14 does cause hyperinnervation. By creating chicks with nerveless wings, we show that from E7, wound healing in the absence of nerves is significantly impaired. These observations suggest that, from the earliest stages of skin innervation, the presence of nerves is beneficial to the healing process, but that, in contrast to neonatal and adult tissues, wound healing in the embryo and early foetus does not trigger hyperinnervation.

Published

2002

15. In vivo imaging indicates muscle fiber dedifferentiation is a major contributor to the regenerating tail blastema

Author

Karen Echeverri, Jonathan D.W. Clarke, and Elly M. Tanaka

Subjects

Tail, Cell type, Time Factors, Microinjections, Muscle Fibers, Skeletal, Ambystoma, Models, Biological, Axolotl, Multinucleate, Dermis, medicine, Myocyte, Animals, Regeneration, blastema, Molecular Biology, Cell Nucleus, biology, Regeneration (biology), Cartilage, Muscles, dedifferentiation, Cell Differentiation, Dextrans, Cell Biology, Anatomy, biology.organism_classification, Cell biology, Ambystoma mexicanum, muscle fibers, medicine.anatomical_structure, Microscopy, Fluorescence, Blastema, Developmental Biology

Abstract

During tail regeneration in urodele amphibians such as axolotls, all of the tissue types, including muscle, dermis, spinal cord, and cartilage, are regenerated. It is not known how this diversity of cell types is reformed with such precision. In particular, the number and variety of mature cell types in the remaining stump that contribute to the blastema is unclear. Using Nomarski imaging, we followed the process of regeneration in the larval axolotl tail. Combining this with in vivo fluorescent labeling of single muscle fibers, we show that mature muscle dedifferentiates. Muscle dedifferentiation occurs by the synchronous fragmentation of the multinucleate muscle fiber into mononucleate cells followed by rapid cell proliferation and the extension of cell processes. We further show that direct clipping of the muscle fiber and severe tissue damage around the fiber are both required to initiate dedifferentiation. Our observations also make it possible to estimate for the first time how many of the blastema cells arise specifically from muscle dedifferentiation. Calculations based on our data suggest that up to 29% of nondermal-derived cells in the blastema come from dedifferentiation of mature muscle fibers. Overall, these results show that endogenous multinucleate muscle fibers can dedifferentiate into mononucleate cells and contribute significantly to the blastema.

Published

2001

16. Differential patterning of ventral midline cells by axial mesoderm is regulated by BMP7 and chordin

Author

Jonathan D.W. Clarke, Jane Dodd, Marysia Placzek, N. Sattar, J. Heemskerk, and K. Dale

Subjects

Mesoderm, Prechordal plate, animal structures, Embryo, Nonmammalian, Bone Morphogenetic Protein 7, Embryonic Development, Chick Embryo, Biology, FGF and mesoderm formation, Cell Movement, Transforming Growth Factor beta, Notochord, medicine, Paraxial mesoderm, Animals, Hedgehog Proteins, RNA, Messenger, Molecular Biology, In Situ Hybridization, Body Patterning, Glycoproteins, Lateral plate mesoderm, Gene Expression Regulation, Developmental, Proteins, Cell Differentiation, Anatomy, Immunohistochemistry, Cell biology, medicine.anatomical_structure, Spinal Cord, embryonic structures, Bone Morphogenetic Proteins, Microscopy, Electron, Scanning, Trans-Activators, Intercellular Signaling Peptides and Proteins, NODAL, Intermediate mesoderm, Developmental Biology, Signal Transduction

Abstract

Ventral midline cells in the neural tube have distinct properties at different rostrocaudal levels, apparently in response to differential signalling by axial mesoderm. Floor plate cells are induced by sonic hedgehog (SHH) secreted from the notochord whereas ventral midline cells of the rostral diencephalon (RDVM cells) appear to be induced by the dual actions of SHH and bone morphogenetic protein 7 (BMP7) from prechordal mesoderm. We have examined the cellular and molecular events that govern the program of differentiation of RDVM cells under the influence of the axial mesoderm. By fate mapping, we show that prospective RDVM cells migrate rostrally within the neural plate, passing over rostral notochord before establishing register with prechordal mesoderm at stage 7. Despite the co-expression of SHH and BMP7 by rostral notochord, prospective RDVM cells appear to be specified initially as caudal ventral midline neurectodermal cells and to acquire RDVM properties only at stage 7. We provide evidence that the signalling properties of axial mesoderm over this period are regulated by the BMP antagonist, chordin. Chordin is expressed throughout the axial mesoderm as it extends, but is downregulated in prechordal mesoderm coincident with the onset of RDVM cell differentiation. Addition of chordin to conjugate explant cultures of prechordal mesoderm and neural tissue prevents the rostralization of ventral midline cells by prechordal mesoderm. Chordin may thus act to refine the patterning of the ventral midline along the rostrocaudal axis.

Published

1998

17. Dorso-ventral ectodermal compartments and origin of apical ectodermal ridge in developing chick limb

Author

Muriel Altabef, Jonathan D.W. Clarke, and Cheryll Tickle

Subjects

Apical ectodermal ridge, Embryonic Induction, Mesoderm, animal structures, Genes, Homeobox, Ectoderm, Extremities, Anatomy, Chick Embryo, Biology, Models, Biological, Limb bud, medicine.anatomical_structure, Zone of polarizing activity, embryonic structures, medicine, Eye development, Limb development, Compartment (development), Animals, Molecular Biology, Developmental Biology, Signal Transduction

Abstract

We wish to understand how limbs are positioned with respect to the dorso-ventral axis of the body in vertebrate embryos, and how different regions of limb bud ectoderm, i.e. dorsal ectoderm, apical ridge and ventral ectoderm, originate. Signals from dorsal and ventral ectoderm control dorso-ventral patterning while the apical ectodermal ridge (AER) controls bud outgrowth and patterning along the proximo-distal axis. We show, using cell-fate tracers, the existence of two distinct ectodermal compartments, dorsal versus ventral, in both presumptive limb and flank of early chick embryos. This organisation of limb ectoderm is the first direct evidence, in vertebrates, of compartments in non-neural ectoderm. Since the apical ridge appears to be confined to this compartment boundary, this positions the limb. The mesoderm, unlike the ectoderm, does not contain two separate dorsal and ventral cell lineages, suggesting that dorsal and ventral ectoderm compartments may be important to ensure appropriate control of mesodermal cell fate. Surprisingly, we also show that cells which form the apical ridge are initially scattered in a wide region of early ectoderm and that both dorsal and ventral ectoderm cells contribute to the apical ridge, intermingling to some extent within it.

Published

1997

18. Relationship between dose, distance and time in Sonic Hedgehog-mediated regulation of anteroposterior polarity in the chick limb

Author

Delphine Duprez, Yingzi Yang, Pao-Tien Chuang, Neil Vargesson, David Bumcrot, Cheryll Tickle, Jonathan D.W. Clarke, Elisa Martí, G Drossopoulou, Lee Niswander, and Andrew P. McMahon

Subjects

animal structures, Body Patterning, Mesenchyme, Chick Embryo, Limb bud, medicine, Animals, Wings, Animal, Hedgehog Proteins, Sonic hedgehog, Molecular Biology, Regulation of gene expression, biology, Dose-Response Relationship, Drug, Cell Membrane, Gene Expression Regulation, Developmental, Proteins, Transfection, Anatomy, Recombinant Proteins, Cell biology, medicine.anatomical_structure, Zone of polarizing activity, embryonic structures, CD4 Antigens, COS Cells, biology.protein, Trans-Activators, Signal transduction, Developmental Biology, Signal Transduction

Abstract

Anteroposterior polarity in the vertebrate limb is thought to be regulated in response to signals derived from a specialized region of distal posterior mesenchyme, the zone of polarizing activity. Sonic Hedgehog (Shh) is expressed in the zone of polarizing activity and appears to mediate the action of the zone of polarizing activity. Here we have manipulated Shh signal in the limb to assess whether it acts as a longrange signal to directly pattern all the digits. Firstly, we demonstrate that alterations in digit development are dependent upon the dose of Shh applied. DiI-labeling experiments indicate that cells giving rise to the extra digits lie within a 300 μm radius of a Shh bead and that the most posterior digits come from cells that lie very close to the bead. A response to Shh involves a 12-16 hour period in which no irreversible changes in digit pattern occur. Increasing the time of exposure to Shh leads to specification of additional digits, firstly digit 2, then 3, then 4. Cell marking experiments demonstrate that cells giving rise to posterior digits are first specified as anterior digits and later adopt a more posterior character. To monitor the direct range of Shh signalling, we developed sensitive assays for localizing Shh by attaching alkaline phosphatase to Shh and introducing cells expressing these forms into the limb bud. These experiments demonstrate that long-range diffusion across the anteroposterior axis of the limb is possible. However, despite a dramatic difference in their diffusibility in the limb mesenchyme, the two forms of alkaline phosphatase-tagged Shh proteins share similar polarizing activity. Moreover, Shh-N (aminoterminal peptide of Shh)-coated beads and Shh-expressing cells also exhibit similar patterning activity despite a significant difference in the diffusibility of Shh from these two sources. Finally, we demonstrate that when Shh-N is attached to an integral membrane protein, cells transfected with this anchored signal also induce mirror-image pattern duplications in a dose-dependent fashion similar to the zone of polarizing activity itself. These data suggest that it is unlikely that Shh itself signals digit formation at a distance. Beads soaked in Shh-N do not induce Shh in anterior limb mesenchyme ruling out direct propagation of a Shh signal. However, Shh induces dose-dependent expression of Bmp genes in anterior mesenchyme at the start of the promotion phase. Taken together, these results argue that the dose-dependent effects of Shh in the regulation of anteroposterior pattern in the limb may be mediated by some other signal(s). BMPs are plausible candidates.

Published

1997

19. Cell movements, neuronal organisation and gene expression in hindbrains lacking morphological boundaries

Author

David G. Wilkinson, Ronald Nittenberg, Cheryll Tickle, Jonathan D.W. Clarke, Ketan Patel, Robb Krumlauf, Paul M. Brickell, and Yogish Joshi

Subjects

Retinoic acid, Rhombomere, Hindbrain, Tretinoin, Chick Embryo, Biology, chemistry.chemical_compound, Cell Movement, Precursor cell, Animals, Hox gene, Molecular Biology, Early Growth Response Protein 2, Boundary cell, Regulation of gene expression, Embryonic Induction, Homeodomain Proteins, Motor Neurons, Neurons, Neuropeptides, Cranial Nerves, Receptor, EphA4, Gene Expression Regulation, Developmental, Receptor Protein-Tyrosine Kinases, Anatomy, Cell biology, DNA-Binding Proteins, Rhombencephalon, chemistry, embryonic structures, Developmental Biology, Transcription Factors

Abstract

Rhombomeres are segmental units of the hindbrain that are separated from each other by a specialised zone of boundary cells. Retinoic acid application to a recently segmented hindbrain leads to disappearance of posterior rhombomere boundaries. Boundary loss is preceded by changes in segmental expression of Krox-20 and Cek-8 and followed by alterations in Hox gene expression. The characteristic morphology of boundary cells, their expression of follistatin and the periodic accumulation of axons normally associated with boundaries are all lost. In the absence of boundaries, we detect no change in anteroposterior dispersal of precursor cells and, in most cases, no substantial cell mixing between former rhombomeric units. This is consistent with the idea that lineage restriction can be maintained by processes other than a mechanical barrier composed of boundary cells. Much of the early organisation of the motor nuclei appears normal despite the loss of boundaries and altered Hox expression.

Published

1997

20. Retinoic acid causes abnormal development and segmental patterning of the anterior hindbrain in Xenopus embryos

Author

David G. Wilkinson, Jonathan D.W. Clarke, Robb Krumlauf, Nancy Papalopulu, Leila C. Bradley, and Nigel Holder

Subjects

medicine.medical_specialty, animal structures, Embryo, Nonmammalian, Xenopus, Central nervous system, Rhombomere, Retinoic acid, Gene Expression, Hindbrain, Tretinoin, chemistry.chemical_compound, Internal medicine, medicine, Morphogenesis, Animals, Molecular Biology, Zebrafish, biology, Dose-Response Relationship, Drug, Embryogenesis, Gastrula, biology.organism_classification, Cell biology, Gastrulation, Rhombencephalon, Endocrinology, medicine.anatomical_structure, Phenotype, chemistry, Genes, Microscopy, Fluorescence, embryonic structures, Developmental Biology

Abstract

Retinoic acid is a very potent teratogen and has also been implicated as an endogenous developmental signalling molecule in vertebrate embryos. One of the regions of the embryo reliably affected by exogenously applied RA is the hindbrain. In this paper, we describe in detail the hindbrain of Xenopus laevis embryos briefly treated with various levels of RA at gastrula stages. Such treatments lead to development of embryos with loss of anterior structures. In addition, RA has a general effect on rhombomere morphology and specific effects on the development of the anterior rhombomeres. This effect is demonstrated using neurofilament antibodies, HRP staining and in situ hybridisation using a probe for expression of the Xenopus Krox-20 gene. Anatomically it is evident that the development of the hindbrain normally anterior to the otocyst (rhombomeres 1-4) is abnormal following RA treatment. Sensory and motor axons of cranial nerves V and Vll form a single root and the peripheral paths of V and VH and IX and X are also abnormal, as is the more anterior location of the otocyst. These anatomical changes are accompanied by changes in the pattern of expression for the gene XKrox-20, which normally expresses in rhombomeres 3 and 5, but is found in a single band in the anterior hindbrain of treated embryos which standardly fail to generate the normal external segmental appearance. The results are discussed in terms of both the teratogenic and possible endogenous roles of RA during normal development of the central nervous system. We conclude that low doses of RA applied during gastrulation have specific effects on the anterior Xenopus hindbrain which appear to be evolutionarily conserved in the light of similar recent findings in zebrafish.

Published

1991

21. Neuroanatomical and functional analysis of neural tube formation in notochordless Xenopus embryos; laterality of the ventral spinal cord is lost

Author

J. Storm-Mathisen, Jonathan D.W. Clarke, Nigel Holder, and S.R. Soffe

Subjects

Central Nervous System, Motor Neurons, Cord, Central nervous system, Notochord, Anatomy, Motor neuron, Biology, Spinal cord, Immunohistochemistry, Axons, Electrophysiology, Microscopy, Electron, Xenopus laevis, medicine.anatomical_structure, Neurulation, nervous system, Spinal Cord, Ventral nerve cord, medicine, Animals, Molecular Biology, Developmental Biology, Floor plate

Abstract

Notochordless Xenopus embryos were produced by u.v. irradiation of the uncleaved fertilized egg. The spinal cords were examined using intermediate filament staining for glial cells, retrograde HRP staining for neuronal morphology and an anti-glycinergic antibody to reveal commissural cells and axons. The floorplate cells of the normal cord appear to be absent and their position along the ventral midline of the cord is occupied by motor neurones, Kolmer-Agduhr cells, radial glial cells and a ventrally placed marginal zone containing the longitudinal axons. Motor neurone number is reduced to 15 % of control values, and the sensory extramedullary cell number is increased twentyfold. Commissural axons are still able to cross the ventral cord but do so at abnormal angles and some commissural axons continue to grow circumferentially up the contralateral side of the cord rather than turning to grow longitudinally. Extracellular electrophysiological recordings from motor axons reveal that the normal alternation of locomotor activity on the left and right side of the embryo is lost in notochordless animals. These results suggest that the notochord and/or the normal floor plate structure are important for the development of the laterality of spinal cord connections and may influence motor neurone proliferation or differentiation.

Published

1991

22. Progenitor Dispersal and the Origin of Early Neuronal Phenotypes in the Chick Embryo Spinal Cord

Author

Jonathan D.W. Clarke, Ketan Patel, and Lynda Erskine

Subjects

Cell type, Time Factors, Cellular differentiation, Chick Embryo, Biology, 03 medical and health sciences, 0302 clinical medicine, Cell Movement, medicine, Animals, Paired Box Transcription Factors, Cell Lineage, Progenitor cell, PAX3 Transcription Factor, Molecular Biology, Body Patterning, Fluorescent Dyes, 030304 developmental biology, Neurons, 0303 health sciences, Stem Cells, Neural tube, Cell Differentiation, Cell Biology, Anatomy, Carbocyanines, Spinal cord, Cell biology, DNA-Binding Proteins, Neuroepithelial cell, Phenotype, medicine.anatomical_structure, Spinal Cord, Biological dispersal, Neural plate, 030217 neurology & neurosurgery, Transcription Factors, Developmental Biology

Abstract

Using DiI and fluorescent dextrans, we have created fate maps of the neural plate and early neural tube describing the extent of progenitor cell dispersal and the spatial origin of morphologically distinct neuronal cell types along the dorsoventral axis of the developing chick spinal cord. Nonuniform dispersal and mixing of progenitors occur within the early neuroepithelium, with the degree of dispersal being determined by the initial position of the cells along the mediolateral axis of the neural plate. Dispersal is greatest in the midregions of the ventricular epithelium and decreases toward the dorsal and ventral midlines. Phenotypically diverse classes of neurons are born at specific dorsoventral locations in the neural tube. Motor neurons are the most ventral cell type generated followed, at progressively more dorsal positions, by distinct classes of interneurons. Several genes show dorsoventrally restricted patterns of expression within the neural tube and the fate maps were used to investigate the relationship between one of these genes, Pax3, and progenitor cell dispersal and fate. The results indicate that the dorsoventral pattern of Pax3 expression is not maintained by restrictions to cell mixing and are consistent with a role for this transcription factor in specifying the identity of neurons with contralateral descending axons.

23. Cell fate in the chick limb bud and relationship to gene expression

Author

Neil Vargesson, Katherine Vincent, Clare Coles, Cheryll Tickle, Lewis Wolpert, and Jonathan D.W. Clarke

Subjects

Apical ectodermal ridge, Mesoderm, Limb Buds, Mesenchyme, Fibroblast Growth Factor 4, Pyridinium Compounds, Chick Embryo, Biology, Cell fate determination, Limb bud, Proto-Oncogene Proteins, Ectoderm, medicine, Limb development, Animals, Wings, Animal, Molecular Biology, Body Patterning, Fluorescent Dyes, Homeodomain Proteins, Gene Expression Regulation, Developmental, Anatomy, Carbocyanines, Fibroblast Growth Factors, medicine.anatomical_structure, Zone of polarizing activity, Ridge (meteorology), Developmental Biology, Transcription Factors

Abstract

We have produced detailed fate maps for mesenchyme and apical ridge of a stage 20 chick wing bud. The fate maps of the mesenchyme show that most of the wing arises from the posterior half of the bud. Subapical mesenchyme gives rise to digits. Cell populations beneath the ridge in the mid apical region fan out into the anterior tip of the handplate, while posterior cell populations extend right along the posterior margin. Subapical mesenchyme of the leg bud behaves similarly. The absence of anterior bending of posterior cell populations has implications when considering models of vertebrate limb evolution. The fatemaps of the apical ridge show that there is also a marked anterior expansion and cells that were in anterior apical ridge later become incorporated into non-ridge ectoderm along the margin of the bud. Mesenchyme and apical ridge do not expand in concert - the apical ridge extends more anteriorly. We used the fatemaps to investigate the relation-ship between cell lineage and elaboration of Hoxd-13 and Fgf-4 domains. Hoxd-13 and Fgf-4 are initially expressed posteriorly until about the mid-point of the early wing bud in mesenchyme and apical ridge respectively. Later in development, the genes come to be expressed throughout most of the handplate and apical ridge respectively. We found that at the proximal edge of the Hoxd-13 domain, cell populations stopped expressing the gene as development proceeded and found no evidence that the changes in extent of the domains were due to initiation of gene expression in anterior cells. Instead the changes in extent of expression fit with the fate maps and can be attributed to expansion and fanning out of cell populations initially expressing the genes.