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11. N-terminal ataxin-3 causes neurological symptoms with inclusions, endoplasmic reticulum stress and ribosomal dislocation.

Author

Hübener J, Vauti F, Funke C, Wolburg H, Ye Y, Schmidt T, Wolburg-Buchholz K, Schmitt I, Gardyan A, Driessen S, Arnold HH, Nguyen HP, Riess O, Hübener, Jeannette, Vauti, Franz, Funke, Claudia, Wolburg, Hartwig, Ye, Yihong, Schmidt, Thorsten, and Wolburg-Buchholz, Karen

Abstract

Mutant ataxin-3 is aberrantly folded and proteolytically cleaved in spinocerebellar ataxia type 3. The C-terminal region of the protein includes a polyglutamine stretch that is expanded in spinocerebellar ataxia type 3. Here, we report on the analysis of an ataxin-3 mutant mouse that has been obtained by gene trap integration. The ataxin-3 fusion protein encompasses 259 N-terminal amino acids including the Josephin domain and an ubiquitin-interacting motif but lacks the C-terminus with the polyglutamine stretch, the valosin-containing protein binding region and part of the ubiquitin-interacting motif 2. Homozygous ataxin-3 mutant mice were viable and showed no apparent anatomical defects at birth. However, at the age of 9 months, homozygous and heterozygous mutant mice revealed significantly altered behaviour and progressing deficits of motor coordination followed by premature death at ∼12 months. At this time, prominent extranuclear protein aggregates and neuronal cell death was found in mutant mice. This was associated with disturbances of the endoplasmic reticulum-mediated unfolded protein response, consistent with the normal role of ataxin-3 in endoplasmic reticulum homeostasis. Thus, the ataxin-3 gene trap model provides evidence for a contribution of the non-polyglutamine containing ataxin-3 N-terminus, which mimics a calpain fragment that has been observed in spinocerebellar ataxia type 3. Consistent with the disease in humans, gene trap mice develop cytoplasmic inclusion bodies and implicate impaired unfolded protein response in the pathogenesis of spinocerebellar ataxia type 3. [ABSTRACT FROM AUTHOR]

Published
2011
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16. Subcellular relocalization and nuclear redistribution of the RNA methyltransferases TRMT1 and TRMT1L upon neuronal activation.

Author

Jonkhout N, Cruciani S, Santos Vieira HG, Tran J, Liu H, Liu G, Pickford R, Kaczorowski D, Franco GR, Vauti F, Camacho N, Abedini SS, Najmabadi H, Ribas de Pouplana L, Christ D, Schonrock N, Mattick JS, and Novoa EM

Subjects
Animals, Female, Mice, Mice, Knockout, Neuroblastoma genetics, Neuroblastoma metabolism, Neurons cytology, tRNA Methyltransferases genetics, Brain metabolism, Cell Nucleus metabolism, Neuroblastoma pathology, Neurons metabolism, Subcellular Fractions metabolism, tRNA Methyltransferases metabolism
Abstract

RNA modifications are dynamic chemical entities that expand the RNA lexicon and regulate RNA fate. The most abundant modification present in mRNAs, N6-methyladenosine (m 6 A), has been implicated in neurogenesis and memory formation. However, whether additional RNA modifications may be playing a role in neuronal functions and in response to environmental queues is largely unknown. Here we characterize the biochemical function and cellular dynamics of two human RNA methyltransferases previously associated with neurological dysfunction, TRMT1 and its homolog, TRMT1- like (TRMT1L). Using a combination of next-generation sequencing, LC-MS/MS, patient-derived cell lines and knockout mouse models, we confirm the previously reported dimethylguanosine (m 2,2 G) activity of TRMT1 in tRNAs, as well as reveal that TRMT1L, whose activity was unknown, is responsible for methylating a subset of cytosolic tRNA Ala (AGC) isodecoders at position 26. Using a cellular in vitro model that mimics neuronal activation and long term potentiation, we find that both TRMT1 and TRMT1L change their subcellular localization upon neuronal activation. Specifically, we observe a major subcellular relocalization from mitochondria and other cytoplasmic domains (TRMT1) and nucleoli (TRMT1L) to different small punctate compartments in the nucleus, which are as yet uncharacterized. This phenomenon does not occur upon heat shock, suggesting that the relocalization of TRMT1 and TRMT1L is not a general reaction to stress, but rather a specific response to neuronal activation. Our results suggest that subcellular relocalization of RNA modification enzymes may play a role in neuronal plasticity and transmission of information, presumably by addressing new targets.

Published
2021
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17. Structural Analysis and Spatiotemporal Expression of Atxn1 Genes in Zebrafish Embryos and Larvae.

Author

Vauti F, Vögele V, Deppe I, Hahnenstein ST, and Köster RW

Subjects
Animals, Ataxin-1 metabolism, Cerebellum metabolism, Gene Expression genetics, Gene Expression Regulation, Developmental genetics, Larva metabolism, Nerve Tissue Proteins metabolism, Nuclear Proteins metabolism, Phylogeny, Spatio-Temporal Analysis, Spinocerebellar Ataxias genetics, Structure-Activity Relationship, Zebrafish embryology, Zebrafish metabolism, Zebrafish Proteins metabolism, Ataxin-1 genetics, Ataxin-1 physiology
Abstract

Zebrafish have come into focus to model cerebellar diseases such as spinocerebellar ataxias (SCAs), which is caused by an expansion of translated CAG repeats in several unrelated genes. In spinocerebellar ataxia type 1 (SCA1), gain-of-function in the mutant ATXN1 contributes to SCA1's neuropathy. Human ATXN1 and its paralog ATXN1L are chromatin-binding factors, act as transcriptional repressors, and have similar expression patterns. However, little is known about atxn1 genes in zebrafish. Recently, two family members, atxn1a and atxn1b , were identified as duplicate orthologs of ATXN1 , as was a txn1l , the ortholog of ATXN1L . In this study, we analyzed the phylogenetic relationship of the atxn1 family members in zebrafish, compared their genetic structures, and verified the predicted transcripts by both RT-PCR and whole-mount in situ hybridization. All three genes, atxn1a , atxn1b , and atxn1l , show overlapping, but also distinct, expression domains during embryonic and larval development. While atxn1a and atxn1l display similar spatiotemporal embryonic expression, atxn1b expression is initiated during the onset of brain development and is predominantly expressed in the cerebellum throughout zebrafish development. These results provide new insights into atxn1 genes and their expression patterns in zebrafish during embryonic and late-larval development and may contribute importantly to future experiments in disease modeling of SCAs.

Published
2021
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18. Induced Arp2/3 Complex Depletion Increases FMNL2/3 Formin Expression and Filopodia Formation.

Author

Dimchev V, Lahmann I, Koestler SA, Kage F, Dimchev G, Steffen A, Stradal TEB, Vauti F, Arnold HH, and Rottner K

Abstract

The Arp2/3 complex generates branched actin filament networks operating in cell edge protrusion and vesicle trafficking. Here we employ a conditional knockout mouse model permitting tissue- or cell-type specific deletion of the murine Actr3 gene (encoding Arp3). A functional Actr3 gene appeared essential for fibroblast viability and growth. Thus, we developed cell lines for exploring the consequences of acute, tamoxifen-induced Actr3 deletion causing near-complete loss of functional Arp2/3 complex expression as well as abolished lamellipodia formation and membrane ruffling, as expected. Interestingly, Arp3-depleted cells displayed enhanced rather than reduced cell spreading, employing numerous filopodia, and showed little defects in the rates of random cell migration. However, both exploration of new space by individual cells and collective migration were clearly compromised by the incapability to efficiently maintain directionality of migration, while the principal ability to chemotax was only moderately affected. Examination of actin remodeling at the cell periphery revealed reduced actin turnover rates in Arp2/3-deficient cells, clearly deviating from previous sequestration approaches. Most surprisingly, induced removal of Arp2/3 complexes reproducibly increased FMNL formin expression, which correlated with the explosive induction of filopodia formation. Our results thus highlight both direct and indirect effects of acute Arp2/3 complex removal on actin cytoskeleton regulation., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2021 Dimchev, Lahmann, Koestler, Kage, Dimchev, Steffen, Stradal, Vauti, Arnold and Rottner.)

Published
2021
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19. All-age whole mount in situ hybridization to reveal larval and juvenile expression patterns in zebrafish.

Author

Vauti F, Stegemann LA, Vögele V, and Köster RW

Subjects
Animals, Embryo, Nonmammalian, Immunohistochemistry, In Situ Hybridization, Larva genetics, Larva growth & development, Models, Animal, Zebrafish genetics, Developmental Biology methods, Embryonic Development genetics, Gene Expression Regulation, Developmental, Zebrafish growth & development
Abstract

The zebrafish Danio rerio is a valuable and common model for scientists in the fields of genetics and developmental biology. Since zebrafish are also amenable to genetic manipulation, modelling of human diseases or behavioral experiments have moved into the focus of zebrafish research. Consequently, gene expression data beyond embryonic and larval stages become more important, yet there is a dramatic knowledge gap of gene expression beyond day four of development. Like in other model organisms, the visualization of spatial and temporal gene expression by whole mount in situ hybridization (ISH) becomes increasingly difficult when zebrafish embryos develop further and hence the growing tissues become dense and less permeable. Here we introduce a modified method for whole mount ISH, which overcomes these penetration and detection problem. The method is an all in one solution that enables the detection and visualization of gene expression patterns up to the late larval stage in a 3D manner without the need for tissue sectioning and offers a valuable extension for whole mount ISH by immunohistochemistry in the zebrafish field., Competing Interests: The authors have declared that no competing interests exist.

Published
2020
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20. Single-Stranded DNA-Binding Transcriptional Regulator FUBP1 Is Essential for Fetal and Adult Hematopoietic Stem Cell Self-Renewal.

Author

Rabenhorst U, Thalheimer FB, Gerlach K, Kijonka M, Böhm S, Krause DS, Vauti F, Arnold HH, Schroeder T, Schnütgen F, von Melchner H, Rieger MA, and Zörnig M

Subjects
Adult Stem Cells cytology, Adult Stem Cells metabolism, Animals, Cell Differentiation genetics, Cell Proliferation genetics, DNA, Single-Stranded genetics, DNA, Single-Stranded metabolism, DNA-Binding Proteins antagonists & inhibitors, Fetal Stem Cells cytology, Fetal Stem Cells metabolism, Gene Expression Regulation, Hematopoiesis genetics, Hematopoietic Stem Cells cytology, Mice, Signal Transduction genetics, Cell Self Renewal genetics, DNA-Binding Proteins genetics, Hematopoietic Stem Cells metabolism
Abstract

The ability of hematopoietic stem cells (HSCs) to self-renew is a prerequisite for the establishment of definitive hematopoiesis and life-long blood regeneration. Here, we report the single-stranded DNA-binding transcriptional regulator far upstream element (FUSE)-binding protein 1 (FUBP1) as an essential factor of HSC self-renewal. Functional inactivation of FUBP1 in two different mouse models resulted in embryonic lethal anemia at around E15.5 caused by severely diminished HSCs. Fetal and adult HSCs lacking FUBP1 revealed an HSC-intrinsic defect in their maintenance, expansion, and long-term blood reconstitution, but could differentiate into all hematopoietic lineages. FUBP1-deficient adult HSCs exhibit significant transcriptional changes, including upregulation of the cell-cycle inhibitor p21 and the pro-apoptotic Noxa molecule. These changes caused an increase in generation time and death of HSCs as determined by video-microscopy-based tracking. Our data establish FUBP1 and its recognition of single-stranded genomic DNA as an important element in the transcriptional regulation of HSC self-renewal., (Copyright © 2015 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2015
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21. Generation of a Nkx2.2(Cre) knock-in mouse line: Analysis of cell lineages in the central nervous system.

Author

Jarrar W, Vauti F, Arnold HH, and Holz A

Subjects
Animals, Body Patterning genetics, Cell Differentiation genetics, Cell Lineage, Central Nervous System growth & development, Gene Expression Regulation, Developmental, Gene Knock-In Techniques, Homeobox Protein Nkx-2.2, Mice, Motor Neurons cytology, Spinal Cord growth & development, Zebrafish Proteins, Central Nervous System cytology, Homeodomain Proteins genetics, Spinal Cord cytology, Transcription Factors genetics
Abstract

A Nkx2.2(cre) knock-in mutant mouse line was generated that on the appropriate reporter strain enables cell fate analysis of the Nkx2.2 cell lineage in the central nervous system and elsewhere. We here demonstrate that Nkx2.2 lineage-marked cells reside in the ventral p3 region along the entire length of the CNS and also in pancreas of mouse embryos. Nkx2.2(+) progenitor cells develop into V3 interneurons in spinal cord and generate the branchio-visceral motor nuclei of cranial nerves in hindbrain. Nkx2.2(+) cells in hindbrain also form serotonergic neurons and oligodendrocytes during later developmental stages. In mouse mutants lacking Nkx2.2 protein the neuronal progenitor cells in spinal cord are transformed to the distinct fate of somatic motor neurons including their axonal projections that exit the CNS ventrally and no longer cross the midline at the commissure. These data identify Nkx2.2 as key regulator to determine neuronal subtypes in the p3 domain of the central nervous system., (Copyright © 2015 International Society of Differentiation. Published by Elsevier B.V. All rights reserved.)

Published
2015
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22. Generation and characterization of a tamoxifen-inducible Eomes(CreER) mouse line.

Author

Pimeisl IM, Tanriver Y, Daza RA, Vauti F, Hevner RF, Arnold HH, and Arnold SJ

Subjects
Alleles, Animals, Female, Liver embryology, Liver metabolism, Male, Mice, Spleen embryology, Spleen metabolism, Integrases genetics, Mice, Transgenic, Models, Animal, T-Box Domain Proteins genetics, Tamoxifen pharmacology
Abstract

Transgenic mouse lines expressing inducible forms of Cre-recombinase in a tissue-specific manner are powerful genetic tools for studying aspects of development and various processes in the adult. The T-box transcription factor eomesodermin (Eomes) plays critical roles for maintenance and differentiation of different pools of stem and progenitor cells from early embryonic stages to adulthood. These include trophoblast stem cells, epiblast cells during the generation of the primary germ layers, neurogenic intermediate progenitor cells in embryonic and adult cortical neurogenesis, and maturing natural killer and T cells. Here, we report on the generation and analysis of an Eomes(CreER) -targeted allele by placing the tamoxifen-activatable Cre-recombinase (CreER) under the control of the Eomes genomic locus. We demonstrate that CreER expression recapitulates endogenous Eomes transcription within different progenitor cell populations. Tamoxifen administration specifically labels Eomes-expressing cells and their progeny as demonstrated by crossing Eomes(CreER) animals to different Cre-inducible reporter strains. In summary, this novel Eomes(CreER) allele can be used as elegant genetic tool that allows to follow the fate of Eomes-positive cells and to genetically manipulate them in a temporal specific manner., (Copyright © 2013 Wiley Periodicals, Inc.)

Published
2013
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23. Popeye domain containing proteins are essential for stress-mediated modulation of cardiac pacemaking in mice.

Author

Froese A, Breher SS, Waldeyer C, Schindler RF, Nikolaev VO, Rinné S, Wischmeyer E, Schlueter J, Becher J, Simrick S, Vauti F, Kuhtz J, Meister P, Kreissl S, Torlopp A, Liebig SK, Laakmann S, Müller TD, Neumann J, Stieber J, Ludwig A, Maier SK, Decher N, Arnold HH, Kirchhof P, Fabritz L, and Brand T

Subjects
Animals, Biological Clocks, Bradycardia genetics, Electrocardiography methods, Electrophysiology methods, Heart Rate, Membrane Proteins metabolism, Mice, Mice, Transgenic, Phenotype, Protein Structure, Tertiary, Telemetry methods, Time Factors, Cell Adhesion Molecules metabolism, Muscle Proteins metabolism, Potassium Channels, Tandem Pore Domain metabolism
Abstract

Cardiac pacemaker cells create rhythmic pulses that control heart rate; pacemaker dysfunction is a prevalent disorder in the elderly, but little is known about the underlying molecular causes. Popeye domain containing (Popdc) genes encode membrane proteins with high expression levels in cardiac myocytes and specifically in the cardiac pacemaking and conduction system. Here, we report the phenotypic analysis of mice deficient in Popdc1 or Popdc2. ECG analysis revealed severe sinus node dysfunction when freely roaming mutant animals were subjected to physical or mental stress. In both mutants, bradyarrhythmia developed in an age-dependent manner. Furthermore, we found that the conserved Popeye domain functioned as a high-affinity cAMP-binding site. Popdc proteins interacted with the potassium channel TREK-1, which led to increased cell surface expression and enhanced current density, both of which were negatively modulated by cAMP. These data indicate that Popdc proteins have an important regulatory function in heart rate dynamics that is mediated, at least in part, through cAMP binding. Mice with mutant Popdc1 and Popdc2 alleles are therefore useful models for the dissection of the mechanisms causing pacemaker dysfunction and could aid in the development of strategies for therapeutic intervention.

Published
2012
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24. Transcriptional regulator BPTF/FAC1 is essential for trophoblast differentiation during early mouse development.

Author

Goller T, Vauti F, Ramasamy S, and Arnold HH

Subjects
Animals, Antigens, Nuclear genetics, Biomarkers metabolism, Cytokines, Embryo, Mammalian anatomy & histology, Fetal Proteins genetics, Fetal Proteins metabolism, Humans, In Situ Hybridization, Mice, Mutation, Nerve Tissue Proteins genetics, Proteins genetics, Proteins metabolism, T-Box Domain Proteins genetics, T-Box Domain Proteins metabolism, Transcription Factors genetics, Trophoblasts cytology, Brachyury Protein, Antigens, Nuclear metabolism, Cell Differentiation physiology, Embryo, Mammalian physiology, Nerve Tissue Proteins metabolism, Transcription Factors metabolism, Transcription, Genetic, Trophoblasts physiology
Abstract

The putative transcriptional regulator BPTF/FAC1 is expressed in embryonic and extraembryonic tissues of the early mouse conceptus. The extraembryonic trophoblast lineage in mammals is essential to form the fetal part of the placenta and hence for the growth and viability of the embryo in utero. Here, we describe a loss-of-function allele of the BPTF/FAC1 gene that causes embryonic lethality in the mouse. BPTF/FAC1-deficient embryos form apparently normal blastocysts that implant and develop epiblast, visceral endoderm, and extraembryonic ectoderm including trophoblast stem cells. Subsequent development of mutants, however, is arrested at the early gastrula stage (embryonic day 6.5), and virtually all null embryos die before midgestation. Most notably, the ectoplacental cone is drastically reduced or absent in mutants, which may cause the embryonic lethality. Development of the mutant epiblast is also affected, as the anterior visceral endoderm and the primitive streak do not form correctly, while brachyury-expressing mesodermal cells arise but are delayed. The mutant phenotype suggests that gastrulation is initiated, but no complete anteroposterior axis of the epiblast appears. We conclude that BPTF/FAC1 is essential in the extraembryonic lineage for correct development of the ectoplacental cone and fetomaternal interactions. In addition, BPTF/FAC1 may also play a role either directly or indirectly in anterior-posterior patterning of the epiblast.

Published
2008
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25. The hnRNP and cytoskeletal protein raver1 contributes to synaptic plasticity.

Author

Lahmann I, Fabienke M, Henneberg B, Pabst O, Vauti F, Minge D, Illenberger S, Jockusch BM, Korte M, and Arnold HH

Subjects
Animals, Cells, Cultured, Cytoskeletal Proteins physiology, Electrophysiology, Embryo, Mammalian, Fibroblasts, Hippocampus, Long-Term Potentiation, Mice, Mice, Knockout, Nuclear Proteins deficiency, Phenotype, RNA-Binding Proteins, Ribonucleoproteins, Carrier Proteins physiology, Heterogeneous-Nuclear Ribonucleoproteins physiology, Neuronal Plasticity, Nuclear Proteins physiology, Synapses physiology
Abstract

Raver1 is an hnRNP protein that interacts with the ubiquitous splicing regulator PTB and binds to cytoskeletal components like alpha-actinin and vinculin/metavinculin. Cell culture experiments suggested that raver1 functions as corepressor in PTB-regulated splicing reactions and may thereby increase proteome complexity. To determine the role of raver1 in vivo, we inactivated the gene by targeted disruption in the mouse. Here we report that raver1-deficient mice develop regularly to adulthood and show no obvious anatomical or behavioral defects. In keeping with this notion, cells from raver1-null mice were indistinguishable from wild type cells and displayed normal growth, motility, and cytoskeletal architecture in culture. Moreover, alternative splicing of exons, including the model exon 3 of alpha-tropomyosin, was not markedly changed in mutant mice, suggesting that the role of raver1 for PTB-mediated exon repression is not absolutely required to generate splice variants during mouse development. Interestingly however, loss of raver1 caused significantly reduced plasticity of synapses on acute hippocampal slices, as elicited by electrophysiological measurements of markedly lower LTP and LTD in mutant neurons. Our results provide evidence that raver1 may play an important role for the regulation of neuronal synaptic plasticity, possibly by controlling especially the late LTP via posttranscriptional mechanisms.

Published
2008
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26. Arp3 is required during preimplantation development of the mouse embryo.

Author

Vauti F, Prochnow BR, Freese E, Ramasamy SK, Ruiz P, and Arnold HH

Subjects
Actin-Related Protein 3 genetics, Animals, Female, Heterozygote, Homozygote, Mice, Mice, Mutant Strains, Models, Genetic, Mutation, Phenotype, Pregnancy, Actin-Related Protein 3 physiology, Blastocyst physiology, Embryonic Development genetics
Abstract

The role of Arp3 in mouse development was investigated utilizing a gene trap mutation in the Arp3 gene. Heterozygous Arp3(WT/GT) mice are normal, however, homozygous Arp3(GT/GT) embryos die at blastocyst stage. Earlier embryonic stages appear unaffected by the mutation, probably due to maternal Arp3 protein. Mutant blastocysts isolated at E3.5 fail to continue development in vitro, lack outgrowth of trophoblast-like cells in culture and express reduced levels of the trophoblast marker Cdx2, while markers for inner cell mass continue to be present. The recessive embryonic lethal phenotype indicates that Arp3 plays a vital role for early mouse development, possibly when trophoblast cells become critical for implantation.

Published
2007
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27. The mouse Trm1-like gene is expressed in neural tissues and plays a role in motor coordination and exploratory behaviour.

Author

Vauti F, Goller T, Beine R, Becker L, Klopstock T, Hölter SM, Wurst W, Fuchs H, Gailus-Durner V, de Angelis MH, and Arnold HH

Subjects
Animals, Cloning, Organism, Embryonic Development, Embryonic Stem Cells metabolism, Female, Male, Mice, Organ Specificity, tRNA Methyltransferases genetics, Brain metabolism, Exploratory Behavior, Motor Activity, Nerve Tissue metabolism, tRNA Methyltransferases metabolism
Abstract

Using a gene trap approach in ES cells, the novel mouse gene Trm1-like with substantial sequence homology to human C1orf25 mRNA (GenBank accession no. ) was identified. Murine Trm1-like encodes a putative protein with limited similarity to N2,N2-dimethylguanosine tRNA methyltransferase (Trm1) from other organisms, however its function is not known. The potential role of Trm1-like was investigated in a mouse mutant lacking intact Trm1-like transcripts due to integration of the gene trap vector in the first intron. Trm1-like deficient mice are viable and show no apparent anatomical defects. Behavioural tests, however, revealed significantly altered motor coordination and aberrant exploratory behaviour. LacZ activity of the trapped mouse Trm1-like gene reflects expression in various neuronal structures during embryonic development, including spinal ganglia, trigeminal nerve and ganglion, olfactory and nasopharyngeal epithelium, and nuclei of the metencephalon, thalamus and medulla oblongata. The gene is also expressed in lung, oesophagus, epiglottis, ependyma, vertebral column, spinal cord, and brown adipose tissue. Trm1-like expression persists in the adult brain with dynamically changing patterns in cortex and cerebellum. Although Trm1-like is not essential for embryonic mouse development, it may have a role in modulating postnatal neuronal functions.

Published
2007
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28. Inactivation of a testis-specific Lis1 transcript in mice prevents spermatid differentiation and causes male infertility.

Author

Nayernia K, Vauti F, Meinhardt A, Cadenas C, Schweyer S, Meyer BI, Schwandt I, Chowdhury K, Engel W, and Arnold HH

Subjects
1-Alkyl-2-acetylglycerophosphocholine Esterase, Acrosome metabolism, Animals, Apoptosis, Blotting, Northern, Blotting, Western, Cell Differentiation, Cell Nucleus metabolism, DNA Fragmentation, Disease Models, Animal, Dyneins biosynthesis, Exons, Female, Gene Library, Genotype, Homozygote, Immunohistochemistry, Male, Mice, Mice, Transgenic, Microscopy, Electron, Models, Genetic, Mutation, Phenotype, Reverse Transcriptase Polymerase Chain Reaction, Spermatogenesis, Tubulin biosynthesis, Infertility, Male etiology, Microtubule-Associated Proteins biosynthesis, Spermatids metabolism, Testis metabolism
Abstract

Lis1 protein is the non-catalytic component of platelet-activating factor acetylhydrolase 1b (PAF-AH 1B) and associated with microtubular structures. Hemizygous mutations of the LIS1 gene cause type I lissencephaly, a brain abnormality with developmental defects of neuronal migration. Lis1 is also expressed in testis, but its function there has not been determined. We have generated a mouse mutant (LIS1GT/GT) by gene trap integration leading to selective disruption of a Lis1 splicing variant in testis. Homozygous mutant males are infertile with no other apparent phenotype. We demonstrate that Lis1 is predominantly expressed in spermatids, and spermiogenesis is blocked when Lis1 is absent. Mutant spermatids fail to form correct acrosomes and nuclei appear distorted in size and shape. The tissue architecture in mutant testis appears severely disturbed displaying collapsed seminiferous tubules, mislocated germ cells, and increased apoptosis. These results provide evidence for an essential and hitherto uncharacterized role of the Lis1 protein in spermatogenesis, particularly in the differentiation of spermatids into spermatozoa.

Published
2003
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29. A large-scale, gene-driven mutagenesis approach for the functional analysis of the mouse genome.

Author

Hansen J, Floss T, Van Sloun P, Füchtbauer EM, Vauti F, Arnold HH, Schnütgen F, Wurst W, von Melchner H, and Ruiz P

Subjects
Animals, Base Sequence, Cell Line, DNA genetics, Genetic Vectors, Humans, Mice, Inbred C57BL, Mice, Transgenic, Phenotype, Sequence Tagged Sites, Stem Cells, Genomics methods, Mice genetics, Mutagenesis, Insertional methods
Abstract

A major challenge of the postgenomic era is the functional characterization of every single gene within the mammalian genome. In an effort to address this challenge, we assembled a collection of mutations in mouse embryonic stem (ES) cells, which is the largest publicly accessible collection of such mutations to date. Using four different gene-trap vectors, we generated 5,142 sequences adjacent to the gene-trap integration sites (gene-trap sequence tags; http://genetrap.de) from >11,000 ES cell clones. Although most of the gene-trap vector insertions occurred randomly throughout the genome, we found both vector-independent and vector-specific integration "hot spots." Because >50% of the hot spots were vector-specific, we conclude that the most effective way to saturate the mouse genome with gene-trap insertions is by using a combination of gene-trap vectors. When a random sample of gene-trap integrations was passaged to the germ line, 59% (17 of 29) produced an observable phenotype in transgenic mice, a frequency similar to that achieved by conventional gene targeting. Thus, gene trapping allows a large-scale and cost-effective production of ES cell clones with mutations distributed throughout the genome, a resource likely to accelerate genome annotation and the in vivo modeling of human disease.

Published
2003
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30. Nephrin TRAP mice lack slit diaphragms and show fibrotic glomeruli and cystic tubular lesions.

Author

Rantanen M, Palmén T, Pätäri A, Ahola H, Lehtonen S, Aström E, Floss T, Vauti F, Wurst W, Ruiz P, Kerjaschki D, and Holthöfer H

Subjects
Animals, Fibrosis, Genotype, Immunohistochemistry, Kidney embryology, Membrane Proteins, Mice, Proteins analysis, Proteins genetics, RNA, Messenger analysis, Kidney ultrastructure, Kidney Glomerulus pathology, Kidney Tubules pathology, Proteins physiology
Abstract

The molecular mechanisms maintaining glomerular filtration barrier are under intensive study. This study describes a mutant Nphs1 mouse line generated by gene-trapping. Nephrin, encoded by Nphs1, is a structural protein of interpodocyte filtration slits crucial for formation of primary urine. Nephrin(trap/trap) mutants show characteristic features of proteinuric disease and die soon after birth. Morphologically, fibrotic glomeruli with distorted structures and cystic tubular lesions were observed, but no prominent changes in the branching morphogenesis of the developing collecting ducts could be found. Western blotting and immunohistochemical analyses confirmed the absence of nephrin in nephrin(trap/trap) glomeruli. The immunohistochemical staining showed also that the interaction partner of nephrin, CD2-associated protein (CD2AP), and the slit-diaphragm-associated protein, ZO-1alpha (-), appeared unchanged, whereas the major anionic apical membrane protein of podocytes, podocalyxin, somewhat punctate as compared with the wild-type (wt) and nephrin(wt/trap) stainings. Electron microscopy revealed that >90% of the podocyte foot processes were fused. The remaining interpodocyte junctions lacked slit diaphragms and, instead, showed tight adhering areas. In the heterozygote glomeruli, approximately one third of the foot processes were fused and real-time RT-PCR showed >60% decrease of nephrin-specific transcripts. These results show an effective nephrin gene elimination, resulting in a phenotype that resembles human congenital nephrotic syndrome. Although the nephrin(trap/trap) mice can be used to study the pathophysiology of the disease, the heterozygous mice may provide a useful model to study the gene dose effect of this crucial protein of the glomerular filtration barrier.

Published
2002
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33. Platelet signal transduction mechanisms induced by eicosanoids.

Author

Siess W, Grünberg B, Luber K, Vauti F, and Wilhelm B

Subjects
Humans, Platelet Activation drug effects, Prostaglandins pharmacology, Thromboxanes pharmacology, Type C Phospholipases metabolism, Blood Platelets metabolism, Eicosanoids pharmacology, Signal Transduction drug effects
Abstract

Platelets are in many ways involved in the pathogenesis of artherosclerosis and the development of coronary heart disease, and play a role in acute myocardial infarction (8). They are also an useful model to study cellular activation mechanisms: their isolation from peripheral venous blood is simple and rapid and their physiological responses such as shape change, aggregation and secretion can be easily measured (10). This chapter is focused on our results on the mechanisms of platelet activation and inhibition induced by eicosanoids.

Published
1992

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