Your search keyword '"Burt, DW"' showing total 4 results

1. Visualisation of chicken macrophages using transgenic reporter genes: insights into the development of the avian macrophage lineage.

Author

Balic A, Garcia-Morales C, Vervelde L, Gilhooley H, Sherman A, Garceau V, Gutowska MW, Burt DW, Kaiser P, Hume DA, and Sang HM

Subjects

Animals, Animals, Genetically Modified, Base Sequence, Birds, Cell Lineage, Chickens, Dendritic Cells cytology, Genes, Reporter, Genetic Techniques, Immune System, Introns, Molecular Sequence Data, Phagocytosis, Receptor, Macrophage Colony-Stimulating Factor metabolism, Sequence Homology, Nucleic Acid, Species Specificity, Transgenes, Yolk Sac physiology, Gene Expression Regulation, Developmental, Macrophages cytology

Abstract

We have generated the first transgenic chickens in which reporter genes are expressed in a specific immune cell lineage, based upon control elements of the colony stimulating factor 1 receptor (CSF1R) locus. The Fms intronic regulatory element (FIRE) within CSF1R is shown to be highly conserved in amniotes and absolutely required for myeloid-restricted expression of fluorescent reporter genes. As in mammals, CSF1R-reporter genes were specifically expressed at high levels in cells of the macrophage lineage and at a much lower level in granulocytes. The cell lineage specificity of reporter gene expression was confirmed by demonstration of coincident expression with the endogenous CSF1R protein. In transgenic birds, expression of the reporter gene provided a defined marker for macrophage-lineage cells, identifying the earliest stages in the yolk sac, throughout embryonic development and in all adult tissues. The reporter genes permit detailed and dynamic visualisation of embryonic chicken macrophages. Chicken embryonic macrophages are not recruited to incisional wounds, but are able to recognise and phagocytose microbial antigens., (© 2014. Published by The Company of Biologists Ltd.)

Published

2014

2. Major transcriptome re-organisation and abrupt changes in signalling, cell cycle and chromatin regulation at neural differentiation in vivo.

Author

Olivera-Martinez I, Schurch N, Li RA, Song J, Halley PA, Das RM, Burt DW, Barton GJ, and Storey KG

Subjects

Animals, Body Patterning, Cell Cycle, Cell Differentiation, Cell Lineage, Chick Embryo, Epigenesis, Genetic, Fibroblast Growth Factors metabolism, Gene Expression Regulation, Developmental, Histone Deacetylase 1 metabolism, Mice, Oligonucleotide Array Sequence Analysis, Sequence Analysis, RNA, Signal Transduction, Spinal Cord embryology, Time Factors, Transforming Growth Factor beta metabolism, Chromatin metabolism, Neurogenesis physiology, Neurons cytology, Transcriptome

Abstract

Here, we exploit the spatial separation of temporal events of neural differentiation in the elongating chick body axis to provide the first analysis of transcriptome change in progressively more differentiated neural cell populations in vivo. Microarray data, validated against direct RNA sequencing, identified: (1) a gene cohort characteristic of the multi-potent stem zone epiblast, which contains neuro-mesodermal progenitors that progressively generate the spinal cord; (2) a major transcriptome re-organisation as cells then adopt a neural fate; and (3) increasing diversity as neural patterning and neuron production begin. Focussing on the transition from multi-potent to neural state cells, we capture changes in major signalling pathways, uncover novel Wnt and Notch signalling dynamics, and implicate new pathways (mevalonate pathway/steroid biogenesis and TGFβ). This analysis further predicts changes in cellular processes, cell cycle, RNA-processing and protein turnover as cells acquire neural fate. We show that these changes are conserved across species and provide biological evidence for reduced proteasome efficiency and a novel lengthening of S phase. This latter step may provide time for epigenetic events to mediate large-scale transcriptome re-organisation; consistent with this, we uncover simultaneous downregulation of major chromatin modifiers as the neural programme is established. We further demonstrate that transcription of one such gene, HDAC1, is dependent on FGF signalling, making a novel link between signals that control neural differentiation and transcription of a core regulator of chromatin organisation. Our work implicates new signalling pathways and dynamics, cellular processes and epigenetic modifiers in neural differentiation in vivo, identifying multiple new potential cellular and molecular mechanisms that direct differentiation., (© 2014. Published by The Company of Biologists Ltd.)

Published

2014

3. The Talpid3 gene (KIAA0586) encodes a centrosomal protein that is essential for primary cilia formation.

Author

Yin Y, Bangs F, Paton IR, Prescott A, James J, Davey MG, Whitley P, Genikhovich G, Technau U, Burt DW, and Tickle C

Subjects

Actins metabolism, Amino Acid Sequence, Animals, Avian Proteins chemistry, Avian Proteins metabolism, Body Patterning, Centrosome ultrastructure, Chick Embryo, Cilia ultrastructure, Computational Biology, Microtubules ultrastructure, Molecular Sequence Data, Mutation genetics, Neural Tube cytology, Neural Tube embryology, Protein Structure, Tertiary, Protein Transport, Sequence Alignment, Subcellular Fractions metabolism, Avian Proteins genetics, Centrosome metabolism, Chickens metabolism, Cilia metabolism, Organogenesis

Abstract

The chicken talpid(3) mutant, with polydactyly and defects in other embryonic regions that depend on hedgehog (Hh) signalling (e.g. the neural tube), has a mutation in KIAA0568. Similar phenotypes are seen in mice and in human syndromes with mutations in genes that encode centrosomal or intraflagella transport proteins. Such mutations lead to defects in primary cilia, sites where Hh signalling occurs. Here, we show that cells of talpid(3) mutant embryos lack primary cilia and that primary cilia can be rescued with constructs encoding Talpid3. talpid(3) mutant embryos also develop polycystic kidneys, consistent with widespread failure of ciliogenesis. Ultrastructural studies of talpid(3) mutant neural tube show that basal bodies mature but fail to dock with the apical cell membrane, are misorientated and almost completely lack ciliary axonemes. We also detected marked changes in actin organisation in talpid(3) mutant cells, which may explain misorientation of basal bodies. KIAA0586 was identified in the human centrosomal proteome and, using an antibody against chicken Talpid3, we detected Talpid3 in the centrosome of wild-type chicken cells but not in mutant cells. Cloning and bioinformatic analysis of the Talpid3 homolog from the sea anemone Nematostella vectensis identified a highly conserved region in the Talpid3 protein, including a predicted coiled-coil domain. We show that this region is required to rescue primary cilia formation and neural tube patterning in talpid(3) mutant embryos, and is sufficient for centrosomal localisation. Thus, Talpid3 is one of a growing number of centrosomal proteins that affect both ciliogenesis and Hh signalling.

Published

2009

4. Expression of ptc and gli genes in talpid3 suggests bifurcation in Shh pathway.

Author

Lewis KE, Drossopoulou G, Paton IR, Morrice DR, Robertson KE, Burt DW, Ingham PW, and Tickle C

Subjects

Animals, Bone Morphogenetic Protein 2, Bone Morphogenetic Proteins genetics, COUP Transcription Factors, Chick Embryo, Chromosome Mapping, DNA-Binding Proteins genetics, Gene Expression Regulation, Developmental, Genes, Lethal, Hedgehog Proteins, In Situ Hybridization, Limb Buds embryology, Membrane Proteins, Mutation, Oncogene Proteins genetics, Patched Receptors, Phenotype, Polymerase Chain Reaction, Polymorphism, Single-Stranded Conformational, Receptors, Cell Surface genetics, Signal Transduction, Tissue Transplantation, Transcription Factors genetics, Zinc Finger Protein GLI1, Proteins genetics, Receptors, G-Protein-Coupled, Receptors, Steroid, Trans-Activators, Transforming Growth Factor beta

Abstract

talpid3 is an embryonic-lethal chicken mutation in a molecularly un-characterised autosomal gene. The recessive, pleiotropic phenotype includes polydactylous limbs with morphologically similar digits. Previous analysis established that hox-D and bmp genes, that are normally expressed posteriorly in the limb bud in response to a localised, posterior source of Sonic Hedgehog (Shh) are expressed symmetrically across the entire anteroposterior axis in talpid3 limb buds. In contrast, Shh expression itself is unaffected. Here we examine expression of patched (ptc), which encodes a component of the Shh receptor, and is probably itself a direct target of Shh signalling, to establish whether talpid3 acts in the Shh pathway. We find that ptc expression is significantly reduced in talpid3 embryos. We also demonstrate that talpid3 function is not required for Shh signal production but is required for normal response to Shh signals, implicating talpid3 in transduction of Shh signals in responding cells. Our analysis of expression of putative components of the Shh pathway, gli1, gli3 and coupTFII shows that genes regulated by Shh are either ectopically expressed or no longer responsive to Shh signals in talpid3 limbs, suggesting possible bifurcation in the Shh pathway. We also describe genetic mapping of gli1, ptc, shh and smoothened in chickens and confirm by co-segregation analysis that none of these genes correspond to talpid3.

Published

1999