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6. Resolving Heart Regeneration by Replacement Histone Profiling.

Author

Goldman JA, Kuzu G, Lee N, Karasik J, Gemberling M, Foglia MJ, Karra R, Dickson AL, Sun F, Tolstorukov MY, and Poss KD

Subjects
Animals, Animals, Genetically Modified, Base Sequence, Binding Sites, Enhancer Elements, Genetic genetics, Gene Expression Regulation, Developmental, Histones genetics, Myocytes, Cardiac cytology, Myocytes, Cardiac metabolism, Nucleotide Motifs genetics, Regeneration genetics, Transcription Factors metabolism, Zebrafish genetics, Zebrafish metabolism, Heart physiology, Histones metabolism, Regeneration physiology, Zebrafish physiology
Abstract

Chromatin regulation is a principal mechanism governing animal development, yet it is unclear to what extent structural changes in chromatin underlie tissue regeneration. Non-mammalian vertebrates such as zebrafish activate cardiomyocyte (CM) division after tissue damage to regenerate lost heart muscle. Here, we generated transgenic zebrafish expressing a biotinylatable H3.3 histone variant in CMs and derived cell-type-specific profiles of histone replacement. We identified an emerging program of putative enhancers that revise H3.3 occupancy during regeneration, overlaid upon a genome-wide reduction of H3.3 from promoters. In transgenic reporter lines, H3.3-enriched elements directed gene expression in subpopulations of CMs. Other elements increased H3.3 enrichment and displayed enhancer activity in settings of injury- and/or Neuregulin1-elicited CM proliferation. Dozens of consensus sequence motifs containing predicted transcription factor binding sites were enriched in genomic regions with regeneration-responsive H3.3 occupancy. Thus, cell-type-specific regulatory programs of tissue regeneration can be revealed by genome-wide H3.3 profiling., (Copyright © 2017 Elsevier Inc. All rights reserved.)

Published
2017
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7. Loss-of-function genetic tools for animal models: cross-species and cross-platform differences.

Author

Housden BE, Muhar M, Gemberling M, Gersbach CA, Stainier DY, Seydoux G, Mohr SE, Zuber J, and Perrimon N

Subjects
Animals, Genotype, Humans, Phenotype, Species Specificity, CRISPR-Cas Systems, Gene Silencing, Models, Animal, Morpholinos pharmacology, Mutagenesis, Mutation genetics, RNA Interference
Abstract

Our understanding of the genetic mechanisms that underlie biological processes has relied extensively on loss-of-function (LOF) analyses. LOF methods target DNA, RNA or protein to reduce or to ablate gene function. By analysing the phenotypes that are caused by these perturbations the wild-type function of genes can be elucidated. Although all LOF methods reduce gene activity, the choice of approach (for example, mutagenesis, CRISPR-based gene editing, RNA interference, morpholinos or pharmacological inhibition) can have a major effect on phenotypic outcomes. Interpretation of the LOF phenotype must take into account the biological process that is targeted by each method. The practicality and efficiency of LOF methods also vary considerably between model systems. We describe parameters for choosing the optimal combination of method and system, and for interpreting phenotypes within the constraints of each method.

Published
2017
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8. Modulation of tissue repair by regeneration enhancer elements.

Author

Kang J, Hu J, Karra R, Dickson AL, Tornini VA, Nachtrab G, Gemberling M, Goldman JA, Black BL, and Poss KD

Subjects
Acetylation, Animal Fins injuries, Animal Fins metabolism, Animals, Animals, Newborn, Cell Proliferation, Chromatin Assembly and Disassembly genetics, Epigenesis, Genetic genetics, Female, Gene Expression Profiling, Gene Expression Regulation genetics, Heart, Histones chemistry, Histones metabolism, Leptin biosynthesis, Leptin genetics, Lysine metabolism, Male, Mice, Myocytes, Cardiac cytology, Promoter Regions, Genetic genetics, Transgenes genetics, Zebrafish Proteins genetics, Enhancer Elements, Genetic genetics, Organ Specificity genetics, Regeneration genetics, Regeneration physiology, Wound Healing genetics, Zebrafish genetics, Zebrafish physiology
Abstract

How tissue regeneration programs are triggered by injury has received limited research attention. Here we investigate the existence of enhancer regulatory elements that are activated in regenerating tissue. Transcriptomic analyses reveal that leptin b (lepb) is highly induced in regenerating hearts and fins of zebrafish. Epigenetic profiling identified a short DNA sequence element upstream and distal to lepb that acquires open chromatin marks during regeneration and enables injury-dependent expression from minimal promoters. This element could activate expression in injured neonatal mouse tissues and was divisible into tissue-specific modules sufficient for expression in regenerating zebrafish fins or hearts. Simple enhancer-effector transgenes employing lepb-linked sequences upstream of pro- or anti-regenerative factors controlled the efficacy of regeneration in zebrafish. Our findings provide evidence for 'tissue regeneration enhancer elements' (TREEs) that trigger gene expression in injury sites and can be engineered to modulate the regenerative potential of vertebrate organs.

Published
2016
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9. Single epicardial cell transcriptome sequencing identifies Caveolin 1 as an essential factor in zebrafish heart regeneration.

Author

Cao J, Navis A, Cox BD, Dickson AL, Gemberling M, Karra R, Bagnat M, and Poss KD

Subjects
Animals, Caveolin 1 genetics, Myocytes, Cardiac cytology, Zebrafish, Zebrafish Proteins genetics, Zebrafish Proteins metabolism, Caveolin 1 metabolism, Heart physiology, Pericardium cytology, Regeneration physiology
Abstract

In contrast to mammals, adult zebrafish have a high capacity to regenerate damaged or lost myocardium through proliferation of cardiomyocytes spared from damage. The epicardial sheet covering the heart is activated by injury and aids muscle regeneration through paracrine effects and as a multipotent cell source, and has received recent attention as a target in cardiac repair strategies. Although it is recognized that epicardium is required for muscle regeneration and itself has high regenerative potential, the extent of cellular heterogeneity within epicardial tissue is largely unexplored. Here, we performed transcriptome analysis on dozens of epicardial lineage cells purified from zebrafish harboring a transgenic reporter for the pan-epicardial gene tcf21. Hierarchical clustering analysis suggested the presence of at least three epicardial cell subsets defined by expression signatures. We validated many new pan-epicardial and epicardial markers by alternative expression assays. Additionally, we explored the function of the scaffolding protein and main component of caveolae, caveolin 1 (cav1), which was present in each epicardial subset. In BAC transgenic zebrafish, cav1 regulatory sequences drove strong expression in ostensibly all epicardial cells and in coronary vascular endothelial cells. Moreover, cav1 mutant zebrafish generated by genome editing showed grossly normal heart development and adult cardiac anatomy, but displayed profound defects in injury-induced cardiomyocyte proliferation and heart regeneration. Our study defines a new platform for the discovery of epicardial lineage markers, genetic tools, and mechanisms of heart regeneration., (© 2016. Published by The Company of Biologists Ltd.)

Published
2016
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10. Nerves Regulate Cardiomyocyte Proliferation and Heart Regeneration.

Author

Mahmoud AI, O'Meara CC, Gemberling M, Zhao L, Bryant DM, Zheng R, Gannon JB, Cai L, Choi WY, Egnaczyk GF, Burns CE, Burns CG, MacRae CA, Poss KD, and Lee RT

Subjects
Animals, Animals, Genetically Modified, Animals, Newborn, Cell Proliferation drug effects, Denervation, Gene Expression Regulation drug effects, Immunity drug effects, Immunity genetics, Inflammation genetics, Mice, Models, Biological, Molecular Sequence Data, Nerve Growth Factor pharmacology, Neuregulin-1 pharmacology, Synaptic Transmission drug effects, Vagotomy, Zebrafish, Cholinergic Neurons physiology, Heart innervation, Heart physiology, Myocytes, Cardiac cytology, Regeneration drug effects
Abstract

Some organisms, such as adult zebrafish and newborn mice, have the capacity to regenerate heart tissue following injury. Unraveling the mechanisms of heart regeneration is fundamental to understanding why regeneration fails in adult humans. Numerous studies have revealed that nerves are crucial for organ regeneration, thus we aimed to determine whether nerves guide heart regeneration. Here, we show using transgenic zebrafish that inhibition of cardiac innervation leads to reduction of myocyte proliferation following injury. Specifically, pharmacological inhibition of cholinergic nerve function reduces cardiomyocyte proliferation in the injured hearts of both zebrafish and neonatal mice. Direct mechanical denervation impairs heart regeneration in neonatal mice, which was rescued by the administration of neuregulin 1 (NRG1) and nerve growth factor (NGF) recombinant proteins. Transcriptional analysis of mechanically denervated hearts revealed a blunted inflammatory and immune response following injury. These findings demonstrate that nerve function is required for both zebrafish and mouse heart regeneration., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published
2015
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11. Nrg1 is an injury-induced cardiomyocyte mitogen for the endogenous heart regeneration program in zebrafish.

Author

Gemberling M, Karra R, Dickson AL, and Poss KD

Subjects
Animals, Cardiomegaly pathology, Cell Proliferation, Echocardiography, Heart Ventricles pathology, Hyperplasia, Myocardium metabolism, Myocardium pathology, Myocytes, Cardiac metabolism, Myocytes, Cardiac pathology, Signal Transduction, Heart physiology, Mitogens metabolism, Neuregulin-1 metabolism, Regeneration, Zebrafish physiology, Zebrafish Proteins metabolism
Abstract

Heart regeneration is limited in adult mammals but occurs naturally in adult zebrafish through the activation of cardiomyocyte division. Several components of the cardiac injury microenvironment have been identified, yet no factor on its own is known to stimulate overt myocardial hyperplasia in a mature, uninjured animal. In this study, we find evidence that Neuregulin1 (Nrg1), previously shown to have mitogenic effects on mammalian cardiomyocytes, is sharply induced in perivascular cells after injury to the adult zebrafish heart. Inhibition of Erbb2, an Nrg1 co-receptor, disrupts cardiomyocyte proliferation in response to injury, whereas myocardial Nrg1 overexpression enhances this proliferation. In uninjured zebrafish, the reactivation of Nrg1 expression induces cardiomyocyte dedifferentiation, overt muscle hyperplasia, epicardial activation, increased vascularization, and causes cardiomegaly through persistent addition of wall myocardium. Our findings identify Nrg1 as a potent, induced mitogen for the endogenous adult heart regeneration program.

Published
2015
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12. The zebrafish as a model for complex tissue regeneration.

Author

Gemberling M, Bailey TJ, Hyde DR, and Poss KD

Subjects
Animals, Models, Animal, Zebrafish genetics, Animal Fins physiology, Brain physiology, Heart physiology, Regeneration, Retina physiology, Spinal Cord physiology
Abstract

For centuries, philosophers and scientists have been fascinated by the principles and implications of regeneration in lower vertebrate species. Two features have made zebrafish an informative model system for determining mechanisms of regenerative events. First, they are highly regenerative, able to regrow amputated fins, as well as a lesioned brain, retina, spinal cord, heart, and other tissues. Second, they are amenable to both forward and reverse genetic approaches, with a research toolset regularly updated by an expanding community of zebrafish researchers. Zebrafish studies have helped identify new mechanistic underpinnings of regeneration in multiple tissues and, in some cases, have served as a guide for contemplating regenerative strategies in mammals. Here, we review the recent history of zebrafish as a genetic model system for understanding how and why tissue regeneration occurs., (Copyright © 2013 Elsevier Ltd. All rights reserved.)

Published
2013
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13. An injury-responsive gata4 program shapes the zebrafish cardiac ventricle.

Author

Gupta V, Gemberling M, Karra R, Rosenfeld GE, Evans T, and Poss KD

Subjects
Animals, Animals, Genetically Modified genetics, Animals, Genetically Modified growth & development, Animals, Genetically Modified metabolism, GATA Transcription Factors genetics, Heart Ventricles cytology, Heart Ventricles growth & development, Morphogenesis, Myocytes, Cardiac cytology, Zebrafish metabolism, Zebrafish Proteins genetics, GATA Transcription Factors metabolism, Heart Ventricles metabolism, Myocytes, Cardiac metabolism, Zebrafish genetics, Zebrafish growth & development, Zebrafish Proteins metabolism
Abstract

A common principle of tissue regeneration is the reactivation of previously employed developmental programs. During zebrafish heart regeneration, cardiomyocytes in the cortical layer of the ventricle induce the transcription factor gene gata4 and proliferate to restore lost muscle. A dynamic cellular mechanism initially creates this cortical muscle in juvenile zebrafish, where a small number of internal cardiomyocytes breach the ventricular wall and expand upon its surface. Here, we find that emergent juvenile cortical cardiomyocytes induce expression of gata4 in a manner similar to during regeneration. Clonal analysis indicates that these cardiomyocytes make biased contributions to build the ventricular wall, whereas gata4(+) cardiomyocytes have little or no proliferation hierarchy during regeneration. Experimental microinjuries or conditions of rapid organismal growth stimulate production of ectopic gata4(+) cortical muscle, implicating biomechanical stress in morphogenesis of this tissue and revealing clonal plasticity. Induced transgenic inhibition defined an essential role for Gata4 activity in morphogenesis of the cortical layer and the preservation of normal cardiac function in growing juveniles, and again in adults during heart regeneration. Our experiments uncover an injury-responsive program that prevents heart failure in juveniles by fortifying the ventricular wall, one that is reiterated in adults to promote regeneration after cardiac damage., (Copyright © 2013 Elsevier Ltd. All rights reserved.)

Published
2013
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14. In vivo monitoring of cardiomyocyte proliferation to identify chemical modifiers of heart regeneration.

Author

Choi WY, Gemberling M, Wang J, Holdway JE, Shen MC, Karlstrom RO, and Poss KD

Subjects
Animals, Animals, Genetically Modified embryology, Animals, Genetically Modified metabolism, Animals, Genetically Modified physiology, Biomarkers metabolism, Catechols pharmacology, Cell Count, Cyclohexylamines pharmacology, Embryo, Nonmammalian cytology, Embryo, Nonmammalian drug effects, Embryo, Nonmammalian physiology, Female, Heart embryology, Hedgehog Proteins agonists, Hedgehog Proteins genetics, Hedgehog Proteins metabolism, Isoquinolines pharmacology, Male, Myocytes, Cardiac drug effects, Myocytes, Cardiac metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Signal Transduction, Thiophenes pharmacology, Transforming Growth Factor beta genetics, Transforming Growth Factor beta metabolism, Transgenes, Ubiquitination, Zebrafish genetics, Zebrafish injuries, Zebrafish physiology, Cell Proliferation, Heart physiology, High-Throughput Screening Assays methods, Myocytes, Cardiac cytology, Regeneration
Abstract

Adult mammalian cardiomyocytes have little capacity to proliferate in response to injury, a deficiency that underlies the poor regenerative ability of human hearts after myocardial infarction. By contrast, zebrafish regenerate heart muscle after trauma by inducing proliferation of spared cardiomyocytes, providing a model for identifying manipulations that block or enhance these events. Although direct genetic or chemical screens of heart regeneration in adult zebrafish present several challenges, zebrafish embryos are ideal for high-throughput screening. Here, to visualize cardiomyocyte proliferation events in live zebrafish embryos, we generated transgenic zebrafish lines that employ fluorescent ubiquitylation-based cell cycle indicator (FUCCI) technology. We then performed a chemical screen and identified several small molecules that increase or reduce cardiomyocyte proliferation during heart development. These compounds act via Hedgehog, Insulin-like growth factor or Transforming growth factor β signaling pathways. Direct examination of heart regeneration after mechanical or genetic ablation injuries indicated that these pathways are activated in regenerating cardiomyocytes and that they can be pharmacologically manipulated to inhibit or enhance cardiomyocyte proliferation during adult heart regeneration. Our findings describe a new screening system that identifies molecules and pathways with the potential to modify heart regeneration.

Published
2013
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15. The regenerative capacity of zebrafish reverses cardiac failure caused by genetic cardiomyocyte depletion.

Author

Wang J, Panáková D, Kikuchi K, Holdway JE, Gemberling M, Burris JS, Singh SP, Dickson AL, Lin YF, Sabeh MK, Werdich AA, Yelon D, Macrae CA, and Poss KD

Subjects
Animals, Cell Death, Heart physiology, Heart Failure genetics, Heart Failure pathology, Myocytes, Cardiac cytology, Regeneration, Zebrafish genetics, Zebrafish physiology
Abstract

Natural models of heart regeneration in lower vertebrates such as zebrafish are based on invasive surgeries causing mechanical injuries that are limited in size. Here, we created a genetic cell ablation model in zebrafish that facilitates inducible destruction of a high percentage of cardiomyocytes. Cell-specific depletion of over 60% of the ventricular myocardium triggered signs of cardiac failure that were not observed after partial ventricular resection, including reduced animal exercise tolerance and sudden death in the setting of stressors. Massive myocardial loss activated robust cellular and molecular responses by endocardial, immune, epicardial and vascular cells. Destroyed cardiomyocytes fully regenerated within several days, restoring cardiac anatomy, physiology and performance. Regenerated muscle originated from spared cardiomyocytes that acquired ultrastructural and electrophysiological characteristics of de-differentiation and underwent vigorous proliferation. Our study indicates that genetic depletion of cardiomyocytes, even at levels so extreme as to elicit signs of cardiac failure, can be reversed by natural regenerative capacity in lower vertebrates such as zebrafish.

Published
2011
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16. Combinatorial binding of transcription factors in the pluripotency control regions of the genome.

Author

Ferraris L, Stewart AP, Kang J, DeSimone AM, Gemberling M, Tantin D, and Fairbrother WG

Subjects
Animals, Binding Sites genetics, Blotting, Western, Cells, Cultured, Chromatin Immunoprecipitation, Chromosome Mapping, Electrophoresis, Polyacrylamide Gel, Gene Expression Regulation, Developmental, High-Throughput Nucleotide Sequencing, Homeodomain Proteins metabolism, Humans, Octamer Transcription Factor-1 metabolism, Octamer Transcription Factor-3 metabolism, Promoter Regions, Genetic, Protein Binding genetics, SOXB1 Transcription Factors genetics, SOXB1 Transcription Factors metabolism, Genome, Homeodomain Proteins genetics, Octamer Transcription Factor-1 genetics, Octamer Transcription Factor-3 genetics
Abstract

The pluripotency control regions (PluCRs) are defined as genomic regions that are bound by POU5F1, SOX2, and NANOG in vivo. We utilized a high-throughput binding assay to record more than 270,000 different DNA/protein binding measurements along incrementally tiled windows of DNA within these PluCRs. This high-resolution binding map is then used to systematically define the context of POU factor binding, and reveals patterns of cooperativity and competition in the pluripotency network. The most prominent pattern is a pervasive binding competition between POU5F1 and the forkhead transcription factors. Like many transcription factors, POU5F1 is co-expressed with a paralog, POU2F1, that shares an apparently identical binding specificity. By analyzing thousands of binding measurements, we discover context effects that discriminate POU2F1 from POU5F1 binding. Proximal NANOG binding promotes POU5F1 binding, whereas nearby SOX2 binding favors POU2F1. We demonstrate by cross-species comparison and by chromatin immunoprecipitation (ChIP) that the contextual sequence determinants learned in vitro are sufficient to predict POU2F1 binding in vivo.

Published
2011
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17. A general mechanism for transcription regulation by Oct1 and Oct4 in response to genotoxic and oxidative stress.

Author

Kang J, Gemberling M, Nakamura M, Whitby FG, Handa H, Fairbrother WG, and Tantin D

Subjects
Amino Acid Sequence, Animals, Dimerization, HeLa Cells, Humans, Inverted Repeat Sequences genetics, Mice, Models, Molecular, Molecular Sequence Data, Mutation, Octamer Transcription Factor-1 chemistry, Octamer Transcription Factor-1 genetics, Octamer Transcription Factor-3 chemistry, Octamer Transcription Factor-3 genetics, Phosphorylation, Protein Binding, Protein Structure, Tertiary, DNA Damage physiology, Gene Expression Regulation, Octamer Transcription Factor-1 metabolism, Octamer Transcription Factor-3 metabolism, Oxidative Stress physiology
Abstract

Oct1 and Oct4 are homologous transcription factors with similar DNA-binding specificities. Here we show that Oct1 is dynamically phosphorylated in vivo following exposure of cells to oxidative and genotoxic stress. We further show that stress regulates the selectivity of both proteins for specific DNA sequences. Mutation of conserved phosphorylation target DNA-binding domain residues in Oct1, and Oct4 confirms their role in regulating binding selectivity. Using chromatin immunoprecipitation, we show that association of Oct4 and Oct1 with a distinct group of in vivo targets is inducible by stress, and that Oct1 is essential for a normal post-stress transcriptional response. Finally, using an unbiased Oct1 target screen we identify a large number of genes targeted by Oct1 specifically under conditions of stress, and show that several of these inducible Oct1 targets are also inducibly bound by Oct4 in embryonic stem cells following stress exposure.

Published
2009
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18. High-throughput biochemical analysis of in vivo location data reveals novel distinct classes of POU5F1(Oct4)/DNA complexes.

Author

Tantin D, Gemberling M, Callister C, and Fairbrother WG

Subjects
Animals, Binding Sites, Cell Line, Chromatin Immunoprecipitation, DNA chemistry, DNA metabolism, Embryonic Stem Cells metabolism, Genomics, Humans, Mice, Oligonucleotide Probes, Promoter Regions, Genetic, Electrophoretic Mobility Shift Assay methods, Octamer Transcription Factor-3 metabolism, Oligonucleotide Array Sequence Analysis methods, Regulatory Elements, Transcriptional
Abstract

The transcription factor POU5F1 is a key regulator of embryonic stem (ES) cell pluripotency and a known oncoprotein. We have developed a novel high-throughput binding assay called MEGAshift (microarray evaluation of genomic aptamers by shift) that we use to pinpoint the exact location, affinity, and stoichiometry of the DNA-protein complexes identified by chromatin immunoprecipitation studies. We consider all genomic regions identified as POU5F1-ChIP-enriched in both human and mouse. Compared with regions that are ChIP-enriched in a single species, we find these regions more likely to be near actively transcribed genes in ES cells. We resynthesize these genomic regions as a pool of tiled 35-mers. This oligonucleotide pool is then assayed for binding to recombinant POU5F1 by gel shift. The degree of binding for each oligonucleotide is accurately measured on a custom oligonucleotide microarray. We explore the relationship between experimentally determined and computationally predicted binding strengths, find many novel functional combinations of POU5F1 half sites, and demonstrate efficient motif discovery by incorporating binding information into a motif finding algorithm. In addition to further refining location studies for transcription factors, this method holds promise for the high-throughput screening of promoters, SNP regions, and epigenetic modifications for factor binding.

Published
2008
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