Your search keyword '"Marcus P S, Dekens"' showing total 17 results

1. A Rapid, Highly Sensitive and Open-Access SARS-CoV-2 Detection Assay for Laboratory and Home Testing

Author

Max J. Kellner, James J. Ross, Jakob Schnabl, Marcus P. S. Dekens, Martin Matl, Robert Heinen, Irina Grishkovskaya, Benedikt Bauer, Johannes Stadlmann, Luis Menéndez-Arias, Andrew D. Straw, Robert Fritsche-Polanz, Marianna Traugott, Tamara Seitz, Alexander Zoufaly, Manuela Födinger, Christoph Wenisch, Johannes Zuber, Vienna COVID-19 Detection Initiative (VCDI), Andrea Pauli, and Julius Brennecke

Subjects

COVID-19 diagnostics, RT-LAMP, coronavirus, SARS-CoV-2, isothermal amplification, open-source, Biology (General), QH301-705.5

Abstract

RT-qPCR-based diagnostic tests play important roles in combating virus-caused pandemics such as Covid-19. However, their dependence on sophisticated equipment and the associated costs often limits their widespread use. Loop-mediated isothermal amplification after reverse transcription (RT-LAMP) is an alternative nucleic acid detection method that overcomes these limitations. Here, we present a rapid, robust, and sensitive RT-LAMP-based SARS-CoV-2 detection assay. Our 40-min procedure bypasses the RNA isolation step, is insensitive to carryover contamination, and uses a colorimetric readout that enables robust SARS-CoV-2 detection from various sample types. Based on this assay, we have increased sensitivity and scalability by adding a nucleic acid enrichment step (Bead-LAMP), developed a version for home testing (HomeDip-LAMP), and identified open-source RT-LAMP enzymes that can be produced in any molecular biology laboratory. On a dedicated website, rtlamp.org (DOI: 10.5281/zenodo.6033689), we provide detailed protocols and videos. Our optimized, general-purpose RT-LAMP assay is an important step toward population-scale SARS-CoV-2 testing.

Published

2022

2. Instrument design and protocol for the study of light controlled processes in aquatic organisms, and its application to examine the effect of infrared light on zebrafish.

Author

Marcus P S Dekens, Nicholas S Foulkes, and Kristin Tessmar-Raible

Subjects

Medicine, Science

Abstract

The acquisition of reliable data strongly depends on experimental design. When studying the effects of light on processes such as behaviour and physiology it is crucial to maintain all environmental conditions constant apart from the one under study. Furthermore, the precise values of the environmental factors applied during the experiment should be known. Although seemingly obvious, these conditions are often not met when the effects of light are being studied. Here, we document and discuss the wavelengths and light intensities of natural and artificial light sources. We present standardised experimental protocols together with building plans of a custom made instrument designed to accurately control light and temperature for experiments using fresh water or marine species. Infrared light is commonly used for recording behaviour and in electrophysiological experiments although the properties of fish photoreceptors potentially allow detection into the far red. As an example of our experimental procedure we have applied our protocol and instrument to specifically test the impact of infrared light (840 nm) on the zebrafish circadian clock, which controls many aspects of behaviour, physiology and metabolism. We demonstrate that infrared light does not influence the zebrafish circadian clock. Our results help to provide a solid framework for the future study of light dependent processes in aquatic organisms.

Published

2017

3. Melanopsin elevates locomotor activity during the wake state of the diurnal zebrafish

Author

Marcus P S Dekens, Bruno M Fontinha, Miguel Gallach, Sandra Pflügler, and Kristin Tessmar‐Raible

Subjects

Mammals, Mice, Rod Opsins, Genetics, Animals, Molecular Biology, Biochemistry, Locomotion, Zebrafish, Melatonin

Abstract

Mammalian and fish pineals play a key role in adapting behaviour to the ambient light conditions through the release of melatonin. In mice, light inhibits nocturnal locomotor activity via the non-visual photoreceptor Melanopsin. In contrast to the extensively studied function of Melanopsin in the indirect regulation of the rodent pineal, its role in the intrinsically photosensitive zebrafish pineal has not been elucidated. Therefore, it is not evident if the light signalling mechanism is conserved between distant vertebrates, and how Melanopsin could affect diurnal behaviour. A double knockout of melanopsins (opn4.1-opn4xb) was generated in the diurnal zebrafish, which manifests attenuated locomotor activity during the wake state. Transcriptome sequencing gave insight into pathways downstream of Melanopsin, implying that sustained repression of the melatonin pathway is required to elevate locomotor activity during the diurnal wake state. Moreover, we show that light induces locomotor activity during the diurnal wake state in an intensity-dependent manner. These observations suggest a common Melanopsin-driven mechanism between zebrafish and mammals, while the diurnal and nocturnal chronotypes are inversely regulated downstream of melatonin.

Published

2022

4. Head-to-head comparison of direct-input RT-PCR and RT-LAMP against RT-qPCR on extracted RNA for rapid SARS-CoV-2 diagnostics

Author

Julius Brennecke, Dominik Handler, Franz Allerberger, Peter Hufnagl, Max J Kellner, Martin Matl, Marcus P. S. Dekens, Julian J Ross, Robert Fritsche-Polanz, Manuela Foedinger, Johannes Zuber, Jakob Schnabl, Alexander Indra, Andrea Pauli, Justine Schaeffer, and Robert Heinen

Subjects

Real-time polymerase chain reaction, Coronavirus disease 2019 (COVID-19), Head to head, business.industry, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), RNA, Medicine, Gold standard (test), Computational biology, business, Systematic testing, Highly sensitive

Abstract

SUMMARYViral pandemics, such as Covid-19, pose serious threats to human societies. To control the spread of highly contagious viruses such as SARS-CoV-2, effective test-trace-isolate strategies require population-wide, systematic testing. Currently, RT-qPCR on extracted RNA is the only broadly accepted test for SARS-CoV-2 diagnostics, which bears the risk of supply chain bottlenecks, often exaggerated by dependencies on proprietary reagents. Here, we directly compare the performance of gold standard diagnostic RT-qPCR on extracted RNA to direct input RT-PCR, RT-LAMP and bead-LAMP on 384 primary patient samples collected from individuals with suspected Covid-19 infection. With a simple five minute crude sample inactivation step and one hour of total reaction time, we achieve assay sensitivities of 98% (direct RT-PCR), 93% (bead-LAMP) and 82% (RT-LAMP) for clinically relevant samples (diagnostic RT-qPCR Ct 98%. For direct RT-PCR, our data further demonstrate a perfect agreement between real-time and end-point measurements, which allow a simple binary classification similar to the powerful visual readout of colorimetric LAMP assays. Our study provides highly sensitive and specific, easy to implement, rapid and cost-effective alternatives to diagnostic RT-qPCR tests.

Published

2021

5. A rapid, highly sensitive and open-access SARS-CoV-2 detection assay for laboratory and home testing

Author

Alexander Zoufaly, Christoph Wenisch, Tamara Seitz, Vienna Covid Diagnostics Initiative, Benedikt Bauer, Johannes Stadlmann, Robert Fritsche-Polanz, Manuela Foedinger, Johannes Zuber, James J. Ross, Marianna Traugott, Andrea Pauli, Jakob Schnabl, Luis Menéndez-Arias, Irina Grishkovskaya, Julius Brennecke, Max J. Kellner, Marcus P. S. Dekens, Robert Heinen, Pauli, Andrea, and Pauli, Andrea [0000-0001-9646-2303]

Subjects

Lysis, business.industry, Computer science, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Embedded system, Home testing, Scalability, Loop-mediated isothermal amplification, Nucleic acid, Assay sensitivity, business, Throughput (business), Highly sensitive

Abstract

Global efforts to combat the Covid-19 pandemic caused by the beta coronavirus SARS-CoV-2 are currently based on RT-qPCR-based diagnostic tests. However, their high cost, moderate throughput and reliance on sophisticated equipment limit widespread implementation. Loop-mediated isothermal amplification after reverse transcription (RT-LAMP) is an alternative detection method that has the potential to overcome these limitations. Here we present a rapid, robust, highly sensitive and versatile RT-LAMP based SARS-CoV-2 detection assay. Our forty-minute procedure bypasses a dedicated RNA isolation step, is insensitive to carry-over contamination, and uses a hydroxynaphthol blue (HNB)-based colorimetric readout, which allows robust SARS-CoV-2 detection from various sample types. Based on this assay, we have substantially increased sensitivity and scalability by a simple nucleic acid enrichment step (bead-LAMP), established a pipette-free version for home testing (HomeDip-LAMP), and developed a version with open source enzymes that can be produced in any molecular biology setting. Our advanced, universally applicable RT-LAMP assay is a major step towards population-scale SARS-CoV-2 testing.

Published

2020

6. A versatile depigmentation, clearing, and labeling method for exploring nervous system diversity

Author

Florian Raible, Hannah Schmidbaur, Saiedeh Saghafi, Marko Pende, Elly M. Tanaka, Oleg Simakov, Alexander W. Stockinger, Karim Vadiwala, Pawel Pasierbek, Prayag Murawala, Marcus P. S. Dekens, Klaus Becker, Roger Revilla-i-Domingo, Sofia-Christina Papadopoulos, Martin Zurl, and Hans-Ulrich Dodt

Subjects

Nervous system, 0303 health sciences, Multidisciplinary, Tissue clearing, biology, Confocal, SciAdv r-articles, Computational biology, In situ hybridization, biology.organism_classification, Mammalian brain, Whole systems, 03 medical and health sciences, 0302 clinical medicine, Depigmentation, medicine.anatomical_structure, medicine, medicine.symptom, Zebrafish, Research Articles, 030217 neurology & neurosurgery, Research Article, Developmental Biology, Neuroscience, 030304 developmental biology

Abstract

A tailored protocol combines pigment removal with clearing, facilitating labeling and whole-body imaging across phylogeny., Tissue clearing combined with deep imaging has emerged as a powerful alternative to classical histological techniques. Whereas current techniques have been optimized for imaging selected nonpigmented organs such as the mammalian brain, natural pigmentation remains challenging for most other biological specimens of larger volume. We have developed a fast DEpigmEntation-Plus-Clearing method (DEEP-Clear) that is easily incorporated in existing workflows and combines whole system labeling with a spectrum of detection techniques, ranging from immunohistochemistry to RNA in situ hybridization, labeling of proliferative cells (EdU labeling) and visualization of transgenic markers. With light-sheet imaging of whole animals and detailed confocal studies on pigmented organs, we provide unprecedented insight into eyes, whole nervous systems, and subcellular structures in animal models ranging from worms and squids to axolotls and zebrafish. DEEP-Clear thus paves the way for the exploration of species-rich clades and developmental stages that are largely inaccessible by regular imaging approaches.

Published

2020

7. Thyrotroph embryonic factor regulates light-induced transcription of repair genes in zebrafish embryonic cells.

Author

Daria Gavriouchkina, Sabine Fischer, Tomi Ivacevic, Jens Stolte, Vladimir Benes, and Marcus P S Dekens

Subjects

Medicine, Science

Abstract

Numerous responses are triggered by light in the cell. How the light signal is detected and transduced into a cellular response is still an enigma. Each zebrafish cell has the capacity to directly detect light, making this organism particularly suitable for the study of light dependent transcription. To gain insight into the light signalling mechanism we identified genes that are activated by light exposure at an early embryonic stage, when specialised light sensing organs have not yet formed. We screened over 14,900 genes using micro-array GeneChips, and identified 19 light-induced genes that function primarily in light signalling, stress response, and DNA repair. Here we reveal that PAR Response Elements are present in all promoters of the light-induced genes, and demonstrate a pivotal role for the PAR bZip transcription factor Thyrotroph embryonic factor (Tef) in regulating the majority of light-induced genes. We show that tefbeta transcription is directly regulated by light while transcription of tefalpha is under circadian clock control at later stages of development. These data leads us to propose their involvement in light-induced UV tolerance in the zebrafish embryo.

Published

2010

8. Instrument design and protocol for the study of light controlled processes in aquatic organisms, and its application to examine the effect of infrared light on zebrafish

Author

Marcus P S, Dekens, Nicholas S, Foulkes, and Kristin, Tessmar-Raible

Subjects

Photoreceptors, Life Cycles, Visible Light, Sensory Receptors, Light, Infrared Rays, Social Sciences, Research and Analysis Methods, Model Organisms, Larvae, Animal Cells, Circadian Clocks, Animals, Psychology, Particle Physics, Zebrafish, Neurons, Photons, Infrared Radiation, Physics, Electromagnetic Radiation, Organisms, Fishes, Biology and Life Sciences, Afferent Neurons, Equipment Design, Animal Models, Cell Biology, Circadian Rhythms, Experimental Organism Systems, Osteichthyes, Cellular Neuroscience, Physical Sciences, Vertebrates, Biological Assay, Sensory Perception, Cellular Types, Chronobiology, Elementary Particles, Research Article, Neuroscience, Signal Transduction, Developmental Biology

Abstract

The acquisition of reliable data strongly depends on experimental design. When studying the effects of light on processes such as behaviour and physiology it is crucial to maintain all environmental conditions constant apart from the one under study. Furthermore, the precise values of the environmental factors applied during the experiment should be known. Although seemingly obvious, these conditions are often not met when the effects of light are being studied. Here, we document and discuss the wavelengths and light intensities of natural and artificial light sources. We present standardised experimental protocols together with building plans of a custom made instrument designed to accurately control light and temperature for experiments using fresh water or marine species. Infrared light is commonly used for recording behaviour and in electrophysiological experiments although the properties of fish photoreceptors potentially allow detection into the far red. As an example of our experimental procedure we have applied our protocol and instrument to specifically test the impact of infrared light (840 nm) on the zebrafish circadian clock, which controls many aspects of behaviour, physiology and metabolism. We demonstrate that infrared light does not influence the zebrafish circadian clock. Our results help to provide a solid framework for the future study of light dependent processes in aquatic organisms.

Published

2016

9. Identification of recessive maternal-effect mutations in the zebrafish using a gynogenesis-based method

Author

Christiane Nüsslein-Volhard, Hans-Martin Maischein, Marcus P. S. Dekens, Catrin Weiler, Francisco Pelegri, and Stefan Schulte-Merker

Subjects

Genetics, Mutation, biology, Mutant, Morphogenesis, Maternal effect, biology.organism_classification, medicine.disease_cause, Phenotype, Forward genetics, medicine, Gene, Zebrafish, Developmental Biology

Abstract

In animal species, early developmental processes are driven by maternally derived factors. Here, we describe a forward genetics approach to identify recessive mutations in genes encoding such maternal factors in the zebrafish. We used a gynogenesis-based approach to identify 14 recessive maternal-effect mutations. Homozygosity for these mutations in adult females leads to the inviability of their offspring. Confocal microscopy of embryos labeled with a DNA dye and a membrane marker allowed us to further analyze mutant embryos for defects in nuclear and cellular divisions. The mutations result in a range of defects in early developmental processes, including egg activation, early nuclear events, mitosis, cytokinesis, axial patterning, and gastrulation. Our effort constitutes a systematic attempt to identify maternal-effect genes in a vertebrate species. The sample of mutations that we have identified reflects the diversity of maternally driven functions in early development and underscores the importance of maternal factors in this process.

Published

2004

10. Light Regulates the Cell Cycle in Zebrafish

Author

Marcus P. S. Dekens, David Whitmore, Daniela Vallone, Cristina Santoriello, Nicholas S. Foulkes, and Gabriele Grassi

Subjects

Cell type, Light, Photoperiod, Circadian clock, Enzyme-Linked Immunosorbent Assay, Biology, General Biochemistry, Genetics and Molecular Biology, Animals, Circadian rhythm, Zebrafish, Cells, Cultured, Agricultural and Biological Sciences(all), Staining and Labeling, Biochemistry, Genetics and Molecular Biology(all), Cell growth, Myocardium, Cell Cycle, Cell cycle, biology.organism_classification, Bacterial circadian rhythms, Circadian Rhythm, Cell biology, Bromodeoxyuridine, Light effects on circadian rhythm, Larva, General Agricultural and Biological Sciences

Abstract

The timing of cell proliferation is a key factor contributing to the regulation of normal growth. Daily rhythms of cell cycle progression have been documented in a wide range of organisms [1, 2]. However, little is known about how environmental, humoral, and cell-autonomous factors contribute to these rhythms. Here, we demonstrate that light plays a key role in cell cycle regulation in the zebrafish. Exposure of larvae to light-dark (LD) cycles causes a range of different cell types to enter S phase predominantly at the end of the day. When larvae are raised in constant darkness (DD), a low level of arrhythmic S phase is observed. In addition, light-entrained cell cycle rhythms persist for several days after transfer to DD, both observations pointing to the involvement of the circadian clock [3–6]. We show that the number of LD cycles experienced is essential for establishing this rhythm during larval development. Furthermore, we reveal that the same phenomenon exists in a zebrafish cell line. This represents the first example of a vertebrate cell culture system where circadian rhythms of the cell cycle are observed. Thus, we implicate the cell-autonomous circadian clock in the regulation of the vertebrate cell cycle by light.

Published

2003

11. cdx4 mutants fail to specify blood progenitors and can be rescued by multiple hox genes

Author

George Q. Daley, Stanley J. Korsmeyer, Marcus P. S. Dekens, James Palis, Leonard I. Zon, Patricia Ernst, Yuan Wang, Paul D. Kingsley, and Alan J. Davidson

Subjects

Cell type, Mesoderm, animal structures, Genotype, Molecular Sequence Data, Cell fate determination, Biology, Kidney, Cell Line, Mice, medicine, Animals, RNA, Messenger, Cloning, Molecular, Hox gene, Zebrafish, Body Patterning, Homeodomain Proteins, Genetics, Multidisciplinary, Embryogenesis, Genes, Homeobox, Gene Expression Regulation, Developmental, Zebrafish Proteins, Hematopoietic Stem Cells, biology.organism_classification, Embryonic stem cell, Hematopoiesis, Haematopoiesis, Phenotype, medicine.anatomical_structure, Multigene Family, Mutation, embryonic structures

Abstract

Organogenesis is dependent on the formation of distinct cell types within the embryo. Important to this process are the hox genes, which are believed to confer positional identities to cells along the anteroposterior axis. Here, we have identified the caudal-related gene cdx4 as the locus mutated in kugelig (kgg), a zebrafish mutant with an early defect in haematopoiesis that is associated with abnormal anteroposterior patterning and aberrant hox gene expression. The blood deficiency in kgg embryos can be rescued by overexpressing hoxb7a or hoxa9a but not hoxb8a, indicating that the haematopoietic defect results from perturbations in specific hox genes. Furthermore, the haematopoietic defect in kgg mutants is not rescued by scl overexpression, suggesting that cdx4 and hox genes act to make the posterior mesoderm competent for blood development. Overexpression of cdx4 during zebrafish development or in mouse embryonic stem cells induces blood formation and alters hox gene expression. Taken together, these findings demonstrate that cdx4 regulates hox genes and is necessary for the specification of haematopoietic cell fate during vertebrate embryogenesis.

Published

2003

12. Thyrotroph embryonic factor regulates light-induced transcription of repair genes in zebrafish embryonic cells

Author

Tomi Ivacevic, Vladimir Benes, Daria Gavriouchkina, Marcus P. S. Dekens, Sabine C. Fischer, and Jens Stolte

Subjects

Light Signal Transduction, DNA Repair, Transcription, Genetic, Ultraviolet Rays, Response element, lcsh:Medicine, Response Elements, Cell Biology/Cell Signaling, Transcription (biology), Transcriptional regulation, Animals, lcsh:Science, Promoter Regions, Genetic, Zebrafish, Transcription factor, Cell Biology/Gene Expression, Early embryonic stage, Multidisciplinary, biology, lcsh:R, Gene Expression Regulation, Developmental, Promoter, Genetics and Genomics/Gene Expression, Zebrafish Proteins, biology.organism_classification, Molecular biology, Basic-Leucine Zipper Transcription Factors, lcsh:Q, THYROTROPH EMBRYONIC FACTOR, DNA Damage, Research Article

Abstract

Numerous responses are triggered by light in the cell. How the light signal is detected and transduced into a cellular response is still an enigma. Each zebrafish cell has the capacity to directly detect light, making this organism particularly suitable for the study of light dependent transcription. To gain insight into the light signalling mechanism we identified genes that are activated by light exposure at an early embryonic stage, when specialised light sensing organs have not yet formed. We screened over 14,900 genes using micro-array GeneChips, and identified 19 light-induced genes that function primarily in light signalling, stress response, and DNA repair. Here we reveal that PAR Response Elements are present in all promoters of the light-induced genes, and demonstrate a pivotal role for the PAR bZip transcription factor Thyrotroph embryonic factor (Tef) in regulating the majority of light-induced genes. We show that tefbeta transcription is directly regulated by light while transcription of tefalpha is under circadian clock control at later stages of development. These data leads us to propose their involvement in light-induced UV tolerance in the zebrafish embryo.

Published

2010

13. Autonomous onset of the circadian clock in the zebrafish embryo

Author

David Whitmore and Marcus P. S. Dekens

Subjects

animal structures, Time Factors, Light, Transcription, Genetic, Period (gene), Circadian clock, CLOCK Proteins, Models, Biological, General Biochemistry, Genetics and Molecular Biology, Article, Oscillometry, Basic Helix-Loop-Helix Transcription Factors, Animals, Circadian rhythm, Oscillating gene, Molecular Biology, Zebrafish, Genetics, General Immunology and Microbiology, ARNTL Transcription Factors, biology, Models, Genetic, General Neuroscience, Temperature, Gene Expression Regulation, Developmental, Zebrafish Proteins, biology.organism_classification, Cell biology, Circadian Rhythm, ARNTL, Trans-Activators, Transcription Factors

Abstract

On the first day of development a circadian clock becomes functional in the zebrafish embryo. How this oscillator is set in motion remains unclear. We demonstrate that zygotic period1 transcription begins independent of light exposure. Pooled embryos maintained in darkness and under constant temperature show elevated non-oscillating levels of period1 expression. Consequently, there is no maternal effect or developmental event that sets the phase of the circadian clock. Analysis of period1 transcription, at the cellular level in the absence of environmental stimuli, reveals oscillations in cells that are asynchronous within the embryo. Demonstrating an autonomous onset to rhythmic period1 expression. Transcription of clock1 and bmal1 is rhythmic in the adult, but constant during development in light-entrained embryos. Transient expression of dominant-negative DeltaCLOCK blocks period1 transcription, thus showing that endogenous CLOCK is essential for the transcriptional regulation of period1 in the embryo. We demonstrate a default mechanism in the embryo that initiates the autonomous onset of the circadian clock. This embryonic clock is differentially regulated from that in the adult, the transition coinciding with the appearance of several clock output processes.

Published

2008

14. Identification of recessive maternal-effect mutations in the zebrafish using a gynogenesis-based method

Author

Francisco, Pelegri, Marcus P S, Dekens, Stefan, Schulte-Merker, Hans-Martin, Maischein, Catrin, Weiler, and Christiane, Nüsslein-Volhard

Subjects

Male, Embryo, Nonmammalian, Phenotype, Mutation, Morphogenesis, Animals, Female, Genes, Recessive, Zebrafish, Body Patterning, Mutagens

Abstract

In animal species, early developmental processes are driven by maternally derived factors. Here, we describe a forward genetics approach to identify recessive mutations in genes encoding such maternal factors in the zebrafish. We used a gynogenesis-based approach to identify 14 recessive maternal-effect mutations. Homozygosity for these mutations in adult females leads to the inviability of their offspring. Confocal microscopy of embryos labeled with a DNA dye and a membrane marker allowed us to further analyze mutant embryos for defects in nuclear and cellular divisions. The mutations result in a range of defects in early developmental processes, including egg activation, early nuclear events, mitosis, cytokinesis, axial patterning, and gastrulation. Our effort constitutes a systematic attempt to identify maternal-effect genes in a vertebrate species. The sample of mutations that we have identified reflects the diversity of maternally driven functions in early development and underscores the importance of maternal factors in this process.

Published

2004

15. The maternal-effect gene futile cycle is essential for pronuclear congression and mitotic spindle assembly in the zebrafish zygote

Author

Christiane Nüsslein-Volhard, Francisco Pelegri, Hans-Martin Maischein, and Marcus P. S. Dekens

Subjects

Centrosome, Zygote, Cell division, Transcription, Genetic, Somatic cell, Cleavage Stage, Ovum, Mitosis, Spindle Apparatus, Cell cycle, Biology, Cleavage (embryo), Spindle pole body, Cell biology, Genes, cdc, Meiosis, Microtubule, Animals, Female, Molecular Biology, Cell Division, Zebrafish, Developmental Biology, Microtubule nucleation

Abstract

Embryos have been successfully used for the general study of the cell cycle. Although there are significant differences between the early embryonic and the somatic cell cycle in vertebrates, the existence of specialised factors that play a role during the early cell cycles has remained elusive. We analysed a lethal recessive maternal-effect mutant, futile cycle(fue), isolated in a maternal-effect screen for nuclear division defects in the zebrafish (Danio rerio). The pronuclei fail to congress in zygotes derived from homozygous fue mothers. In addition,a defect in the formation of chromosomal microtubules prevents mitotic spindle assembly and thus chromosome segregation in fue zygotes. However,centrosomal functions do not appear to be affected in fue embryos,suggesting this mutant blocks a subset of microtubule functions. Cleavage occurs normally for several divisions resulting in many anucleate cells, thus showing that nuclear- and cell division can be uncoupled genetically. Therefore, we propose that in mitotic spindle assembly chromosome-dependent microtubule nucleation is essential for the coupling of nuclear and cell division.

Published

2003

16. A radiation hybrid map of the zebrafish genome

Author

Teresa Nicolson, Gerd-Jörg Rauch, T Roeser, Robert Geisler, Darren Gilmour, Annette Kirn, Alexander F. Schier, U Schönberger, S Glaser, C Seydler, K Hingst, Florian Maderspacher, Carl J. Neumann, C. Fricke, Pascal Haffter, Michael A. Gates, H Habeck, U Martyn, Stephan C.F. Neuhauss, Helia B. Schonthaler, Horst Geiger, K Finger, Stefan Schulte-Merker, Scott A. Holley, Herwig Baier, Russell S. Ray, J Keenan, Francisco Pelegri, L Gnügge, Marcus P. S. Dekens, Henry Roehl, Deval A. Lashkari, Holger Knaut, F. van Bebber, Heike E. Schauerte, Christian Weiler, William S. Talbot, L Bross, Jens M. Rick, Silke Geiger-Rudolph, Christiane Nüsslein-Volhard, University of Zurich, and Geisler, R

Subjects

Genetic Markers, Candidate gene, Positional cloning, Biology, Genome, Sequence-tagged site, Gene mapping, 1311 Genetics, Genetics, Animals, Simple sequence length polymorphism, Zebrafish, Sequence Tagged Sites, Electrophoresis, Agar Gel, Expressed Sequence Tags, Expressed sequence tag, Polymorphism, Genetic, Models, Genetic, Chromosome Mapping, Physical Chromosome Mapping, 10124 Institute of Molecular Life Sciences, Genetic marker, 570 Life sciences, biology, Lod Score, Software

Abstract

Recent large-scale mutagenesis screens have made the zebrafish the first vertebrate organism to allow a forward genetic approach to the discovery of developmental control genes. Mutations can be cloned positionally, or placed on a simple sequence length polymorphism (SSLP) map to match them with mapped candidate genes and expressed sequence tags (ESTs). To facilitate the mapping of candidate genes and to increase the density of markers available for positional cloning, we have created a radiation hybrid (RH) map of the zebrafish genome. This technique is based on somatic cell hybrid lines produced by fusion of lethally irradiated cells of the species of interest with a rodent cell line. Random fragments of the donor chromosomes are integrated into recipient chromosomes or retained as separate minichromosomes. The radiation-induced breakpoints can be used for mapping in a manner analogous to genetic mapping, but at higher resolution and without a need for polymorphism. Genome-wide maps exist for the human, based on three RH panels of different resolutions, as well as for the dog, rat and mouse. For our map of the zebrafish genome, we used an existing RH panel and 1,451 sequence tagged site (STS) markers, including SSLPs, cloned candidate genes and ESTs. Of these, 1,275 (87.9%) have significant linkage to at least one other marker. The fraction of ESTs with significant linkage, which can be used as an estimate of map coverage, is 81.9%. We found the average marker retention frequency to be 18.4%. One cR3000 is equivalent to 61 kb, resulting in a potential resolution of approximately 350 kb.

Published

1999

17. The carp homeobox gene Ovx1 shows early expression during gastrulation and subsequently in the vagal lobe, the facial lobe and the ventral telencephalon

Author

J. Samallo, G. te Kronnie, H.W.J. Stroband, H. Schipper, and Marcus P. S. Dekens

Subjects

Fish Proteins, Telencephalon, Carps, Molecular Sequence Data, In situ hybridization, Biology, Nervous System, Mice, Genetics, medicine, Animals, Humans, Amino Acid Sequence, Carp, In Situ Hybridization, Homeodomain Proteins, Sequence Homology, Amino Acid, Cerebrum, Neural tube, Gene Expression Regulation, Developmental, Anatomy, Gastrula, biology.organism_classification, Lobe, Gastrulation, medicine.anatomical_structure, Homeobox, sense organs, Neural development, Chickens, Developmental Biology

Abstract

The homeobox gene Carp-Ovx1 shows similarity to vertebrate and invertebrate Ovx genes and to Drosophila unplugged. Its expression pattern was studied by in situ hybridization in carp embryos and juveniles. During segmentation, expression becomes gradually limited to the neural tube. In juveniles up to 9 weeks old, cells in the ventral telencephalon, the facial lobe and the vagal lobe show Ovx1 expression, confining expression to parts with chemosensory projections.

Published

1998