Your search keyword '"Samuel, Collombet"' showing total 24 results

1. RSAT 2018: regulatory sequence analysis tools 20th anniversary.

Author

Nga Thi Thuy Nguyen, Bruno Contreras-Moreira, Jaime Abraham Castro-Mondragón, Walter Santana-Garcia, Raul Ossio, Carla Daniela Robles-Espinoza, Mathieu Bahin, Samuel Collombet, Pierre Vincens, Denis Thieffry, Jacques van Helden, Alejandra Medina-Rivera, and Morgane Thomas-Chollier

Published

2018

2. Cooperation, cis-interactions, versatility and evolutionary plasticity of multiple cis-acting elements underlie krox20 hindbrain regulation.

Author

Patrick Torbey, Elodie Thierion, Samuel Collombet, Anne de Cian, Carole Desmarquet-Trin-Dinh, Mathilde Dura, Jean-Paul Concordet, Patrick Charnay, and Pascale Gilardi-Hebenstreit

Subjects

Genetics, QH426-470

Abstract

Cis-regulation plays an essential role in the control of gene expression, and is particularly complex and poorly understood for developmental genes, which are subject to multiple levels of modulation. In this study, we performed a global analysis of the cis-acting elements involved in the control of the zebrafish developmental gene krox20. krox20 encodes a transcription factor required for hindbrain segmentation and patterning, a morphogenetic process highly conserved during vertebrate evolution. Chromatin accessibility analysis reveals a cis-regulatory landscape that includes 6 elements participating in the control of initiation and autoregulatory aspects of krox20 hindbrain expression. Combining transgenic reporter analyses and CRISPR/Cas9-mediated mutagenesis, we assign precise functions to each of these 6 elements and provide a comprehensive view of krox20 cis-regulation. Three important features emerged. First, cooperation between multiple cis-elements plays a major role in the regulation. Cooperation can surprisingly combine synergy and redundancy, and is not restricted to transcriptional enhancer activity (for example, 4 distinct elements cooperate through different modes to maintain autoregulation). Second, several elements are unexpectedly versatile, which allows them to be involved in different aspects of control of gene expression. Third, comparative analysis of the elements and their activities in several vertebrate species reveals that this versatility is underlain by major plasticity across evolution, despite the high conservation of the gene expression pattern. These characteristics are likely to be of broad significance for developmental genes.

Published

2018

3. C/EBPα Activates Pre-existing and De Novo Macrophage Enhancers during Induced Pre-B Cell Transdifferentiation and Myelopoiesis

Author

Chris van Oevelen, Samuel Collombet, Guillermo Vicent, Maarten Hoogenkamp, Cyrille Lepoivre, Aimee Badeaux, Lars Bussmann, Jose Luis Sardina, Denis Thieffry, Miguel Beato, Yang Shi, Constanze Bonifer, and Thomas Graf

Subjects

Medicine (General), R5-920, Biology (General), QH301-705.5

Abstract

Transcription-factor-induced somatic cell conversions are highly relevant for both basic and clinical research yet their mechanism is not fully understood and it is unclear whether they reflect normal differentiation processes. Here we show that during pre-B-cell-to-macrophage transdifferentiation, C/EBPα binds to two types of myeloid enhancers in B cells: pre-existing enhancers that are bound by PU.1, providing a platform for incoming C/EBPα; and de novo enhancers that are targeted by C/EBPα, acting as a pioneer factor for subsequent binding by PU.1. The order of factor binding dictates the upregulation kinetics of nearby genes. Pre-existing enhancers are broadly active throughout the hematopoietic lineage tree, including B cells. In contrast, de novo enhancers are silent in most cell types except in myeloid cells where they become activated by C/EBP factors. Our data suggest that C/EBPα recapitulates physiological developmental processes by short-circuiting two macrophage enhancer pathways in pre-B cells.

Published

2015

4. Krox20 hindbrain regulation incorporates multiple modes of cooperation between cis-acting elements.

Author

Elodie Thierion, Johan Le Men, Samuel Collombet, Céline Hernandez, Fanny Coulpier, Patrick Torbey, Morgane Thomas-Chollier, Daan Noordermeer, Patrick Charnay, and Pascale Gilardi-Hebenstreit

Subjects

Genetics, QH426-470

Abstract

Developmental genes can harbour multiple transcriptional enhancers that act simultaneously or in succession to achieve robust and precise spatiotemporal expression. However, the mechanisms underlying cooperation between cis-acting elements are poorly documented, notably in vertebrates. The mouse gene Krox20 encodes a transcription factor required for the specification of two segments (rhombomeres) of the developing hindbrain. In rhombomere 3, Krox20 is subject to direct positive feedback governed by an autoregulatory enhancer, element A. In contrast, a second enhancer, element C, distant by 70 kb, is active from the initiation of transcription independent of the presence of the KROX20 protein. Here, using both enhancer knock-outs and investigations of chromatin organisation, we show that element C possesses a dual activity: besides its classical enhancer function, it is also permanently required in cis to potentiate the autoregulatory activity of element A, by increasing its chromatin accessibility. This work uncovers a novel, asymmetrical, long-range mode of cooperation between cis-acting elements that might be essential to avoid promiscuous activation of positive autoregulatory elements.

Published

2017

5. Parental-to-embryo switch of chromosome organization in early embryogenesis

Author

Wing Leung, Samuel Collombet, Maud Borensztein, Tarak Shisode, Katia Ancelin, Csilla Várnai, Tristan Piolot, Nicolas Servant, Edith Heard, Rafael Galupa, Takashi Nagano, Peter Fraser, Noémie Ranisavljevic, European Molecular Biology Laboratory [Heidelberg] (EMBL), Génétique et Biologie du Développement, Institut Curie [Paris]-Institut National de la Santé et de la Recherche Médicale (INSERM)-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Université Paris sciences et lettres (PSL), Centre Hospitalier Régional Universitaire [Montpellier] (CHRU Montpellier), Cancer et génome: Bioinformatique, biostatistiques et épidémiologie d'un système complexe, Institut Curie [Paris]-MINES ParisTech - École nationale supérieure des mines de Paris, Université Paris sciences et lettres (PSL)-Université Paris sciences et lettres (PSL)-Institut National de la Santé et de la Recherche Médicale (INSERM), Institut Curie [Paris], and Centre National de la Recherche Scientifique (CNRS)

Subjects

Male, Parents, Embryonic Development, Polycomb-Group Proteins, Biology, Methylation, Histones, Chromosome conformation capture, Genomic Imprinting, Mice, 03 medical and health sciences, Histone H3, 0302 clinical medicine, X Chromosome Inactivation, [SDV.BBM.GTP]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Genomics [q-bio.GN], Animals, Medicine, Chromosome Positioning, [SDV.BDD]Life Sciences [q-bio]/Development Biology, Gene, Alleles, ComputingMilieux_MISCELLANEOUS, Genomic organization, 030304 developmental biology, Epigenomics, Genetics, Regulation of gene expression, 0303 health sciences, Genome, Multidisciplinary, business.industry, Gene Expression Regulation, Developmental, Obstetrics and Gynecology, General Medicine, Chromosomes, Mammalian, Chromatin, Blastocyst, Germ Cells, [SDV.BDD.EO]Life Sciences [q-bio]/Development Biology/Embryology and Organogenesis, Histone, Fertilization, biology.protein, Female, Single-Cell Analysis, business, Genomic imprinting, 030217 neurology & neurosurgery

Abstract

Paternal and maternal epigenomes undergo marked changes after fertilization1. Recent epigenomic studies have revealed the unusual chromatin landscapes that are present in oocytes, sperm and early preimplantation embryos, including atypical patterns of histone modifications2–4 and differences in chromosome organization and accessibility, both in gametes5–8 and after fertilization5,8–10. However, these studies have led to very different conclusions: the global absence of local topological-associated domains (TADs) in gametes and their appearance in the embryo8,9 versus the pre-existence of TADs and loops in the zygote5,11. The questions of whether parental structures can be inherited in the newly formed embryo and how these structures might relate to allele-specific gene regulation remain open. Here we map genomic interactions for each parental genome (including the X chromosome), using an optimized single-cell high-throughput chromosome conformation capture (HiC) protocol12,13, during preimplantation in the mouse. We integrate chromosome organization with allelic expression states and chromatin marks, and reveal that higher-order chromatin structure after fertilization coincides with an allele-specific enrichment of methylation of histone H3 at lysine 27. These early parental-specific domains correlate with gene repression and participate in parentally biased gene expression—including in recently described, transiently imprinted loci14. We also find TADs that arise in a non-parental-specific manner during a second wave of genome assembly. These de novo domains are associated with active chromatin. Finally, we obtain insights into the relationship between TADs and gene expression by investigating structural changes to the paternal X chromosome before and during X chromosome inactivation in preimplantation female embryos15. We find that TADs are lost as genes become silenced on the paternal X chromosome but linger in regions that escape X chromosome inactivation. These findings demonstrate the complex dynamics of three-dimensional genome organization and gene expression during early development. Single-cell allelic HiC analysis, combined with allelic gene expression and chromatin states, reveals parent-of-origin-specific dynamics of chromosome organization and gene expression during mouse preimplantation development.

Published

2020

6. Gene regulation in time and space during x-chromosome inactivation

Author

Agnese Loda, Samuel Collombet, and Edith Heard

Subjects

Male, X Chromosome, X Chromosome Inactivation, Humans, Female, RNA, Long Noncoding, Cell Biology, Gene Silencing, Molecular Biology, Epigenesis, Genetic

Abstract

X-chromosome inactivation (XCI) is the epigenetic mechanism that ensures X-linked dosage compensation between cells of females (XX karyotype) and males (XY). XCI is essential for female embryos to survive through development and requires the accurate spatiotemporal regulation of many different factors to achieve remarkable chromosome-wide gene silencing. As a result of XCI, the active and inactive X chromosomes are functionally and structurally different, with the inactive X chromosome undergoing a major conformational reorganization within the nucleus. In this Review, we discuss the multiple layers of genetic and epigenetic regulation that underlie initiation of XCI during development and then maintain it throughout life, in light of the most recent findings in this rapidly advancing field. We discuss exciting new insights into the regulation of X inactive-specific transcript (XIST), the trigger and master regulator of XCI, and into the mechanisms and dynamics that underlie the silencing of nearly all X-linked genes. Finally, given the increasing interest in understanding the impact of chromosome organization on gene regulation, we provide an overview of the factors that are thought to reshape the 3D structure of the inactive X chromosome and of the relevance of such structural changes for XCI establishment and maintenance.

Published

2022

7. Dynamic reversal of random X-Chromosome inactivation during iPSC reprogramming

Author

San Kit To, Adrian Janiszewski, Irene Talon, Juan Song, Greet Bervoets, Natalie De Geest, Jean-Christophe Marine, Joel Chappell, Florian Rambow, Lotte Vanheer, Caterina Provenzano, Oskar Marín-Béjar, Vincent Pasque, and Samuel Collombet

Subjects

Transcriptional Activation, X Chromosome, Induced Pluripotent Stem Cells, Chromatin silencing, Biology, Histone Deacetylases, X-inactivation, Mice, 03 medical and health sciences, 0302 clinical medicine, Genes, X-Linked, X Chromosome Inactivation, Genetics, Animals, Gene silencing, Gene Silencing, Induced pluripotent stem cell, Genetics (clinical), Tissue homeostasis, 030304 developmental biology, Regulation of gene expression, 0303 health sciences, Research, Cellular Reprogramming, Chromatin, Cell biology, Female, RNA, Long Noncoding, Reprogramming, 030217 neurology & neurosurgery

Abstract

Induction and reversal of chromatin silencing is critical for successful development, tissue homeostasis, and the derivation of induced pluripotent stem cells (iPSCs). X-Chromosome inactivation (XCI) and reactivation (XCR) in female cells represent chromosome-wide transitions between active and inactive chromatin states. Although XCI has long been studied, providing important insights into gene regulation, the dynamics and mechanisms underlying the reversal of stable chromatin silencing of X-linked genes are much less understood. Here, we use allele-specific transcriptomics to study XCR during mouse iPSC reprogramming in order to elucidate the timing and mechanisms of chromosome-wide reversal of gene silencing. We show that XCR is hierarchical, with subsets of genes reactivating early, late, and very late during reprogramming. Early genes are activated before the onset of late pluripotency genes activation. Early genes are located genomically closer to genes that escape XCI, unlike genes reactivating late. Early genes also show increased pluripotency transcription factor (TF) binding. We also reveal that histone deacetylases (HDACs) restrict XCR in reprogramming intermediates and that the severe hypoacetylation state of the inactive X Chromosome (Xi) persists until late reprogramming stages. Altogether, these results reveal the timing of transcriptional activation of monoallelically repressed genes during iPSC reprogramming, and suggest that allelic activation involves the combined action of chromatin topology, pluripotency TFs, and chromatin regulators. These findings are important for our understanding of gene silencing, maintenance of cell identity, reprogramming, and disease. ispartof: Genome Research vol:29 issue:10 pages:1659-1672 ispartof: location:United States status: published

Published

2019

8. RNA polymerase II depletion from the inactive X chromosome territory is not mediated by physical compartmentalization

Author

Gina M. Dailey, Halavatyi A, Edith Heard, Alec Heckert, Samuel Collombet, Claire Dugast-Darzacq, Le Saux A, Xavier Darzacq, and Rall I

Subjects

Regulation of gene expression, biology, Transcription (biology), Chemistry, Heterochromatin, biology.protein, RNA, XIST, RNA polymerase II, Compartmentalization (psychology), Chromatin, Cell biology

Abstract

Sub-nuclear compartmentalization has been proposed to play an important role in gene regulation by segregating active and inactive parts of the genome in distinct physical and biochemical environments, where transcription and epigenetic factors are either concentrated or depleted. The inactive X chromosome offers a paradigm for studying sub-nuclear compartmentalization. When the non-coding Xist RNA coats the X chromosome, it recruits repressors and chromatin factors that trigger gene silencing, and forms a dense body of heterochromatin from which the transcription machinery appears to be excluded. Phase separation has been proposed to be involved in X-chromosome inactivation (XCI) and might explain exclusion of the transcription machinery by preventing its diffusion into the Xist-coated territory. Here, using quantitative fluorescence microscopy and single particle tracking, we show that RNA polymerase II (RNAPII) freely accesses the Xist territory during initiation of XCI, and that its diffusion is not prevented by biophysical constraints. Instead, the apparent depletion of RNAPII is due to the loss of its chromatin bound fraction. These findings demonstrate that initial exclusion of RNA Pol2 from the inactive X is a consequence of its reduced binding rate at the chromatin and gene level, rather than the biophysical compartmentalization of the inactive X heterochromatin domain. The Xist silent compartment is thus a biochemical rather than a biophysical compartment, at least during initiation of XCI.

Published

2021

9. Bioinformatic Analysis of Single-Cell Hi-C Data from Early Mouse Embryo

Author

Yuvia A Pérez-Rico, Katia Ancelin, Samuel Collombet, Nicolas Servant, and Edith Heard

Subjects

0303 health sciences, 03 medical and health sciences, 0302 clinical medicine, medicine.anatomical_structure, Workflow, Cell, medicine, Chromosome Organization, Embryo, Computational biology, Biology, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

The adaptation of Hi-C protocols to enable the investigation of chromosome organization in single cells opens new avenues to study the dynamics of this process during embryogenesis. However, the analysis of single-cell Hi-C data is not yet standardized and raises novel bioinformatic challenges. Here we describe a complete workflow for the analysis of single-cell Hi-C data, with a main focus on allele-specific analysis based on data obtained from hybrid embryos.

Published

2020

10. Bioinformatic Analysis of Single-Cell Hi-C Data from Early Mouse Embryo

Author

Samuel, Collombet, Yuvia A, Pérez-Rico, Katia, Ancelin, Nicolas, Servant, and Edith, Heard

Subjects

Male, Mice, Blastocyst, Cell Cycle, Animals, Computational Biology, Female, Single-Cell Analysis, Embryo, Mammalian, Alleles, Software, Workflow

Abstract

The adaptation of Hi-C protocols to enable the investigation of chromosome organization in single cells opens new avenues to study the dynamics of this process during embryogenesis. However, the analysis of single-cell Hi-C data is not yet standardized and raises novel bioinformatic challenges. Here we describe a complete workflow for the analysis of single-cell Hi-C data, with a main focus on allele-specific analysis based on data obtained from hybrid embryos.

Published

2020

11. Logical modeling of cell fate specification-Application to T cell commitment

Author

Elisabetta, Cacace, Samuel, Collombet, and Denis, Thieffry

Subjects

Thymocytes, Models, Genetic, T-Lymphocytes, Animals, Gene Expression Regulation, Developmental, Cell Differentiation, Computer Simulation, Gene Regulatory Networks, Thymus Gland, Transcription Factors

Abstract

Boolean approaches and extensions thereof are becoming increasingly popular to model signaling and regulatory networks, including those controlling cell differentiation, pattern formation and embryonic development. Here, we describe a logical modeling framework relying on three steps: the delineation of a regulatory graph, the specification of multilevel components, and the encoding of Boolean rules specifying the behavior of model components depending on the levels or activities of their regulators. Referring to a non-deterministic, asynchronous updating scheme, we present several complementary methods and tools enabling the computation of stable activity patterns, the verification of the reachability of such patterns, as well as the generation of mean temporal evolution curves and the computation of the probabilities to reach distinct activity patterns. We apply this logical framework to the regulatory network controlling T lymphocyte specification. This process involves cross-regulations between specific T cell regulatory factors and factors driving alternative differentiation pathways, which remain accessible during the early steps of thymocyte development. Many transcription factors needed for T cell specification are required in other hematopoietic differentiation pathways and are combined in a fine-tuned, time-dependent fashion to achieve T cell commitment. Using the software GINsim, we integrated current knowledge into a dynamical model, which recapitulates the main developmental steps from early progenitors entering the thymus up to T cell commitment, as well as the impact of various documented environmental and genetic perturbations. Our model analysis further enabled the identification of several knowledge gaps. The model, software and whole analysis workflow are provided in computer-readable and executable form to ensure reproducibility and ease extensions.

Published

2020

12. Logical modeling of cell fate specification—Application to T cell commitment

Author

Elisabetta Cacace, Denis Thieffry, and Samuel Collombet

Subjects

Model checking, 0303 health sciences, Theoretical computer science, Process (engineering), Gene regulatory network, computer.file_format, Biology, 03 medical and health sciences, Logical framework, Thymocyte, Workflow, Reachability, Executable, computer, 030304 developmental biology

Abstract

Boolean approaches and extensions thereof are becoming increasingly popular to model signaling and regulatory networks, including those controlling cell differentiation, pattern formation and embryonic development. Here, we describe a logical modeling framework relying on three steps: the delineation of a regulatory graph, the specification of multilevel components, and the encoding of Boolean rules specifying the behavior of model components depending on the levels or activities of their regulators. Referring to a non-deterministic, asynchronous updating scheme, we present several complementary methods and tools enabling the computation of stable activity patterns, the verification of the reachability of such patterns, as well as the generation of mean temporal evolution curves and the computation of the probabilities to reach distinct activity patterns. We apply this logical framework to the regulatory network controlling T lymphocyte specification. This process involves cross-regulations between specific T cell regulatory factors and factors driving alternative differentiation pathways, which remain accessible during the early steps of thymocyte development. Many transcription factors needed for T cell specification are required in other hematopoietic differentiation pathways and are combined in a fine-tuned, time-dependent fashion to achieve T cell commitment. Using the software GINsim, we integrated current knowledge into a dynamical model, which recapitulates the main developmental steps from early progenitors entering the thymus up to T cell commitment, as well as the impact of various documented environmental and genetic perturbations. Our model analysis further enabled the identification of several knowledge gaps. The model, software and whole analysis workflow are provided in computer-readable and executable form to ensure reproducibility and ease extensions.

Published

2020

13. SPEN integrates transcriptional and epigenetic control of X-inactivation

Author

Damarys Loew, François Dossin, Varun Kapoor, Mikael Attia, Julia Roensch, Ye Zhan, Tomasz Chelmicki, Agnes Le Saux, Inês Pinheiro, Jan J. Żylicz, Florent Dingli, Samuel Collombet, Job Dekker, Thomas Mercher, and Edith Heard

Subjects

Male, X Chromosome, Transcription, Genetic, RNA polymerase II, Biology, Methylation, Histone Deacetylases, X-inactivation, Article, Epigenesis, Genetic, Mice, 03 medical and health sciences, 0302 clinical medicine, Protein Domains, X Chromosome Inactivation, Transcription (biology), Animals, Gene Silencing, Promoter Regions, Genetic, Enhancer, Embryonic Stem Cells, 030304 developmental biology, Regulation of gene expression, 0303 health sciences, Multidisciplinary, RNA-Binding Proteins, Embryo, Mammalian, Mi-2/NuRD complex, Chromatin, Cell biology, DNA-Binding Proteins, Blastocyst, Enhancer Elements, Genetic, biology.protein, Female, RNA, Long Noncoding, XIST, 030217 neurology & neurosurgery

Abstract

Xist represents a paradigm for the function of long non-coding RNA in epigenetic regulation, although how it mediates X-chromosome inactivation (XCI) remains largely unexplained. Several proteins that bind to Xist RNA have recently been identified, including the transcriptional repressor SPEN1-3, the loss of which has been associated with deficient XCI at multiple loci2-6. Here we show in mice that SPEN is a key orchestrator of XCI in vivo and we elucidate its mechanism of action. We show that SPEN is essential for initiating gene silencing on the X chromosome in preimplantation mouse embryos and in embryonic stem cells. SPEN is dispensable for maintenance of XCI in neural progenitors, although it significantly decreases the expression of genes that escape XCI. We show that SPEN is immediately recruited to the X chromosome upon the upregulation of Xist, and is targeted to enhancers and promoters of active genes. SPEN rapidly disengages from chromatin upon gene silencing, suggesting that active transcription is required to tether SPEN to chromatin. We define the SPOC domain as a major effector of the gene-silencing function of SPEN, and show that tethering SPOC to Xist RNA is sufficient to mediate gene silencing. We identify the protein partners of SPOC, including NCoR/SMRT, the m6A RNA methylation machinery, the NuRD complex, RNA polymerase II and factors involved in the regulation of transcription initiation and elongation. We propose that SPEN acts as a molecular integrator for the initiation of XCI, bridging Xist RNA with the transcription machinery-as well as with nucleosome remodellers and histone deacetylases-at active enhancers and promoters.

Published

2020

14. ZNF143 protein is an important regulator of the myeloid transcription factor C/EBPα

Author

Kenneth D. Swanson, Elena Levantini, Hanna S. Radomska, Daniel G. Tenen, Alex Ebralidze, Susumu Kobayashi, Min Hee Choi, David Gonzalez, Pu Zhang, Qiling Zhou, Ulrich Steidl, Samuel Collombet, Miroslava Kardosova, Alan D. Friedman, Boris Bartholdy, Annouck Luyten, Meritxell Alberich-Jorda, Gilbert Chong, Linda M. Scott, and Robert S. Welner

Subjects

0301 basic medicine, Transcriptional Activation, Myeloid, Biology, Biochemistry, Cell Line, 03 medical and health sciences, Sp3 transcription factor, CEBPA, medicine, CCAAT-Enhancer-Binding Protein-alpha, CCAAT-enhancer-binding protein (C, Humans, Myeloid Cells, Gene Regulation, Promoter Regions, Genetic, Molecular Biology, STAT4, transcription factor, Conserved Sequence, basic research on transcription factors involved in leukemia, Sp1 transcription factor, promoter, Base Sequence, Myeloid leukemia, Gene Expression Regulation, Developmental, Promoter, Cell Biology, Cell biology, Hematopoiesis, ZNF143, 030104 developmental biology, medicine.anatomical_structure, gene regulation during myeloid differentiation, Trans-Activators, IRF8, Protein Binding

Abstract

The transcription factor C/EBPa is essential for myeloid differentiation and is frequently dysregulated in acute myeloid leukemia. Although studied extensively, the precise regulation of its gene by upstream factors has remained largely elusive. Here, we investigated its transcriptional activation during myeloid differentiation. We identified an evolutionarily conserved octameric sequence, CCCAGCAG, approximate to 100 bases upstream of the CEBPA transcription start site, and demonstrated through mutational analysis that this sequence is crucial for C/EBPa expression. This sequence is present in the genes encoding C/EBPa in humans, rodents, chickens, and frogs and is also present in the promoters of other C/EBP family members. We identified that ZNF143, the human homolog of the Xenopus transcriptional activator STAF, specifically binds to this 8-bp sequence to activate C/EBPa expression in myeloid cells through a mechanism that is distinct from that observed in liver cells and adipocytes. Altogether, our data suggest that ZNF143 plays an important role in the expression of C/EBPa in myeloid cells.

Published

2017

15. Logical modeling of lymphoid and myeloid cell specification and transdifferentiation

Author

Wassim Abou-Jaoudé, Morgane Thomas-Chollier, Samuel Collombet, Bruno Di Stefano, Jose Luis Sardina Ortega, Thomas Graf, Chris van Oevelen, Denis Thieffry, Institut de biologie de l'ENS Paris (IBENS), Centre National de la Recherche Scientifique (CNRS)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Département de Biologie - ENS Paris, École normale supérieure - Paris (ENS Paris), Université Paris sciences et lettres (PSL)-Université Paris sciences et lettres (PSL)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS)-École normale supérieure - Paris (ENS Paris), Université Paris sciences et lettres (PSL)-Université Paris sciences et lettres (PSL)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS), Institut de biologie de l'ENS Paris (UMR 8197/1024) (IBENS), Département de Biologie - ENS Paris, and Université Paris sciences et lettres (PSL)-Université Paris sciences et lettres (PSL)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS)

Subjects

0301 basic medicine, Myeloid, Cellular differentiation, Gene regulatory network, Biology, Sackler Colloquium on Gene Regulatory Networks and Network Models in Development and Evolution, Models, Biological, 03 medical and health sciences, 0302 clinical medicine, medicine, Gene Regulatory Networks, Myeloid Cells, Lymphocytes, Transcription factor, Genetics, B-Lymphocytes, Multidisciplinary, Macrophages, Transdifferentiation, Cell Differentiation, [SDV.BIBS]Life Sciences [q-bio]/Quantitative Methods [q-bio.QM], Cell biology, Haematopoiesis, 030104 developmental biology, medicine.anatomical_structure, Cell Transdifferentiation, Stem cell, Reprogramming, 030217 neurology & neurosurgery

Abstract

International audience; Blood cells are derived from a common set of hematopoietic stem cells, which differentiate into more specific progenitors of the myeloid and lymphoid lineages, ultimately leading to differentiated cells. This developmental process is controlled by a complex regulatory network involving cytokines and their receptors, transcription factors, and chromatin remodelers. Using public data and data from our own molecular genetic experiments (quantitative PCR, Western blot, EMSA) or genome-wide assays (RNA-sequencing, ChIP-sequencing), we have assembled a comprehensive regulatory network encompassing the main transcription factors and signaling components involved in myeloid and lymphoid development. Focusing on B-cell and macrophage development, we defined a qualitative dynamical model recapitulating cytokine-induced differentiation of common progenitors, the effect of various reported gene knockdowns, and the reprogramming of pre-B cells into macrophages induced by the ectopic expression of specific transcription factors. The resulting network model can be used as a template for the integration of new hematopoietic differentiation and transdifferentiation data to foster our understanding of lymphoid/myeloid cell-fate decisions.

Published

2017

16. A Transcription Factor Pulse Can Prime Chromatin for Heritable Transcriptional Memory

Author

Kuo-Kai Chin, Benoit Laurent, Chris van Oevelen, Samuel Collombet, Yang Shi, Denis Thieffry, Thomas Graf, and Aimee Iberg-Badeaux

Subjects

0301 basic medicine, Lipopolysaccharides, Cell division, Transcription, Genetic, Cell, RNA polymerase II, Biology, Methylation, Histones, 03 medical and health sciences, medicine, CCAAT-Enhancer-Binding Protein-alpha, Epigenetics, Molecular Biology, Transcription factor, Gene, Genetics, Lysine, Cell Biology, Chromatin, 030104 developmental biology, medicine.anatomical_structure, Enhancer Elements, Genetic, Gene Expression Regulation, biology.protein, RNA Polymerase II, Chromatin immunoprecipitation, Research Article, Protein Binding, Transcription Factors

Abstract

Short-term and long-term transcriptional memory is the phenomenon whereby the kinetics or magnitude of gene induction is enhanced following a prior induction period. Short-term memory persists within one cell generation or in postmitotic cells, while long-term memory can survive multiple rounds of cell division. We have developed a tissue culture model to study the epigenetic basis for long-term transcriptional memory (LTTM) and subsequently used this model to better understand the epigenetic mechanisms that enable heritable memory of temporary stimuli. We find that a pulse of transcription factor CCAAT/enhancer-binding protein alpha (C/EBPα) induces LTTM on a subset of target genes that survives nine cell divisions. The chromatin landscape at genes that acquire LTTM is more repressed than at those genes that do not exhibit memory, akin to a latent state. We show through chromatin immunoprecipitation (ChIP) and chemical inhibitor studies that RNA polymerase II (Pol II) elongation is important for establishing memory in this model but that Pol II itself is not retained as part of the memory mechanism. More generally, our work reveals that a transcription factor involved in lineage specification can induce LTTM and that failure to rerepress chromatin is one epigenetic mechanism underlying transcriptional memory.

Published

2017

17. Transcription Factors Drive Tet2-Mediated Enhancer Demethylation to Reprogram Cell Fate

Author

Marta Gut, Clara Berenguer, Antonio Gomez, Tian V. Tian, Luciano Di Croce, Denis Thieffry, Bruno Di Stefano, Carolina Segura-Morales, Thomas Graf, Ralph Stadhouders, Jose Luis Sardina, Konrad Hochedlinger, Sergi Aranda, Ivo Gut, Justin Brumbaugh, Samuel Collombet, Simon Heath, and Pulmonary Medicine

Subjects

Male, 0301 basic medicine, DNA Hydroxymethylation, Induced Pluripotent Stem Cells, Biology, Article, Dioxygenases, Kruppel-Like Factor 4, Mice, 03 medical and health sciences, Proto-Oncogene Proteins, Genetics, Animals, Epigenetics, Cells, Cultured, Mice, Knockout, Pioneer factor, Cell Biology, Methylation, DNA Methylation, Fibroblasts, Cellular Reprogramming, Chromatin, Cell biology, DNA-Binding Proteins, Enhancer Elements, Genetic, 030104 developmental biology, DNA methylation, biology.protein, Molecular Medicine, Demethylase, Female, Reprogramming, Transcription Factors

Abstract

Here, we report DNA methylation and hydroxymethylation dynamics at nucleotide resolution using C/EBPα-enhanced reprogramming of B cells into induced pluripotent cells (iPSCs). We observed successive waves of hydroxymethylation at enhancers, concomitant with a decrease in DNA methylation, suggesting active demethylation. Consistent with this finding, ablation of the DNA demethylase Tet2 almost completely abolishes reprogramming. C/EBPα, Klf4, and Tfcp2l1 each interact with Tet2 and recruit the enzyme to specific DNA sites. During reprogramming, some of these sites maintain high levels of 5hmC, and enhancers and promoters of key pluripotency factors become demethylated as early as 1 day after Yamanaka factor induction. Surprisingly, methylation changes precede chromatin opening in distinct chromatin regions, including Klf4 bound sites, revealing a pioneer factor activity associated with alteration in DNA methylation. Rapid changes in hydroxymethylation similar to those in B cells were also observed during compound-accelerated reprogramming of fibroblasts into iPSCs, highlighting the generality of our observations. Using a highly efficient reprogramming system, Sardina et al. examined the dynamics of DNA methylation and hydroxymethylation. They found that throughout the process several transcription factors can recruit Tet2 to specific sites, leading to demethylation. Some of these sites became demethylated before chromatin opening.

Published

2018

18. Constitutively Active SMAD2/3 Are Broad-Scope Potentiators of Transcription-Factor-Mediated Cellular Reprogramming

Author

Tyson, Ruetz, Ulrich, Pfisterer, Bruno, Di Stefano, James, Ashmore, Meryam, Beniazza, Tian V, Tian, Daniel F, Kaemena, Luca, Tosti, Wenfang, Tan, Jonathan R, Manning, Eleni, Chantzoura, Daniella Rylander, Ottosson, Samuel, Collombet, Anna, Johnsson, Erez, Cohen, Kosuke, Yusa, Sten, Linnarsson, Thomas, Graf, Malin, Parmar, and Keisuke, Kaji

Subjects

Induced Pluripotent Stem Cells, Humans, Smad2 Protein, Smad3 Protein, Cellular Reprogramming, Cell Line, Transcription Factors

Abstract

Reprogramming of cellular identity using exogenous expression of transcription factors (TFs) is a powerful and exciting tool for tissue engineering, disease modeling, and regenerative medicine. However, generation of desired cell types using this approach is often plagued by inefficiency, slow conversion, and an inability to produce mature functional cells. Here, we show that expression of constitutively active SMAD2/3 significantly improves the efficiency of induced pluripotent stem cell (iPSC) generation by the Yamanaka factors. Mechanistically, SMAD3 interacts with reprogramming factors and co-activators and co-occupies OCT4 target loci during reprogramming. Unexpectedly, active SMAD2/3 also markedly enhances three other TF-mediated direct reprogramming conversions, from B cells to macrophages, myoblasts to adipocytes, and human fibroblasts to neurons, highlighting broad and general roles for SMAD2/3 as cell-reprogramming potentiators. Our results suggest that co-expression of active SMAD2/3 could enhance multiple types of TF-based cell identity conversion and therefore be a powerful tool for cellular engineering.

Published

2016

19. C/EBPα creates elite cells for iPSC reprogramming by upregulating Klf4 and increasing the levels of Lsd1 and Brd4

Author

Janus S. Jakobsen, Francesco Limone, Bruno Di Stefano, Bo T. Porse, Mirko Francesconi, Matthias Mann, Samuel Collombet, Denis Thieffry, Carolina Segura-Morales, Michael Wierer, Jose Luis Sardina, Thomas Graf, Ralph Stadhouders, and Andreas Lackner

Subjects

0301 basic medicine, Male, Proteomics, Blotting, Western, Induced Pluripotent Stem Cells, Kruppel-Like Transcription Factors, Biology, Cell Line, 03 medical and health sciences, Kruppel-Like Factor 4, Mice, Downregulation and upregulation, CCAAT-Enhancer-Binding Protein-alpha, Animals, Humans, Induced pluripotent stem cell, Cells, Cultured, Histone Demethylases, Induced stem cells, B-Lymphocytes, Reverse Transcriptase Polymerase Chain Reaction, Gene Expression Profiling, HEK 293 cells, Nuclear Proteins, Mouse Embryonic Stem Cells, Cell Biology, Cellular Reprogramming, Cell biology, Up-Regulation, Mice, Inbred C57BL, 030104 developmental biology, Gene Ontology, HEK293 Cells, Cell culture, KLF4, Cancer research, Female, Signal transduction, Reprogramming, Transcription Factors

Abstract

Reprogramming somatic cells into induced pluripotent stem cells (iPSCs) is typically inefficient and has been explained by elite-cell and stochastic models. We recently reported that B cells exposed to a pulse of C/EBPα (Bα' cells) behave as elite cells, in that they can be rapidly and efficiently reprogrammed into iPSCs by the Yamanaka factors OSKM. Here we show that C/EBPα post-transcriptionally increases the abundance of several hundred proteins, including Lsd1, Hdac1, Brd4, Med1 and Cdk9, components of chromatin-modifying complexes present at super-enhancers. Lsd1 was found to be required for B cell gene silencing and Brd4 for the activation of the pluripotency program. C/EBPα also promotes chromatin accessibility in pluripotent cells and upregulates Klf4 by binding to two haematopoietic enhancers. Bα' cells share many properties with granulocyte/macrophage progenitors, naturally occurring elite cells that are obligate targets for leukaemic transformation, whose formation strictly requires C/EBPα.

Published

2015

20. Transcription factor induced reprogramming of B cells

Author

Ralph Stadhouders, Bruno Di Stefano, Ben Lehner, Johanna Goldmann, Jose Luis Sardina, Thomas Graf, Gregoire Stik, Mirko Francesconi, and Samuel Collombet

Subjects

Cancer Research, Genetics, Cell Biology, Hematology, Biology, Molecular Biology, Reprogramming, Transcription factor, Cell biology

Published

2017

21. Time-resolved gene expression profiling during reprogramming of C/EBPα-pulsed B cells into iPS cells

Author

Samuel Collombet, Thomas Graf, and Bruno Di Stefano

Subjects

Statistics and Probability, Data Descriptor, Somatic cell, Cellular differentiation, Induced Pluripotent Stem Cells, Gene Expression, Biology, Library and Information Sciences, Education, Mice, Animals, Induced pluripotent stem cell, B-Lymphocytes, Induced stem cells, Ccaat-enhancer-binding proteins, Microarray analysis techniques, Gene Expression Profiling, Cell Differentiation, Cellular Reprogramming, Microarray Analysis, Molecular biology, Cell biology, Computer Science Applications, Gene expression profiling, CCAAT-Enhancer-Binding Proteins, Statistics, Probability and Uncertainty, Reprogramming, Information Systems

Abstract

The reprogramming of somatic cells to induced pluripotent stem cells (iPSCs) is lengthy and inefficient. The development of a reprogramming system that allows rapid and synchronous reprogramming to pluripotency is imperative for understanding the mechanism of iPSC formation and for future therapeutic applications. We have recently reported that a short expression in mouse primary B cells of the transcription factor C/EBPα before the induction of pluripotency factors increases the iPSC reprogramming efficiency >100-fold, involving 95% of the cells within a week. Here we present a dataset containing the time course of gene expression during this process as determined by microarray and RNA-seq techniques.

Published

2014

22. C/EBPα poises B cells for rapid reprogramming into induced pluripotent stem cells

Author

Chris van Oevelen, Jun Lu, Guillermo P. Vicent, Jose Luis Sardina, Bruno Di Stefano, Denis Thieffry, Miguel Beato, Thomas Graf, Eric M Kallin, and Samuel Collombet

Subjects

Epithelial-Mesenchymal Transition, Induced Pluripotent Stem Cells, Kruppel-Like Transcription Factors, Biology, Dioxygenases, Proto-Oncogene Proteins c-myc, Cytosine, Kruppel-Like Factor 4, Mice, SOX2, Enhancer binding, Proto-Oncogene Proteins, CCAAT-Enhancer-Binding Protein-alpha, Animals, Deoxyribonuclease I, Induced pluripotent stem cell, Transcription factor, Cells, Cultured, B-Lymphocytes, Multidisciplinary, SOXB1 Transcription Factors, Transdifferentiation, DNA Methylation, Cellular Reprogramming, Molecular biology, Chromatin, Up-Regulation, DNA-Binding Proteins, KLF4, Cell Transdifferentiation, Reprogramming, Octamer Transcription Factor-3

Abstract

A pulse of C/EBPα followed by overexpression of the transcription factors Oct4, Sox2, Klf4 and Myc leads to fast and very efficient reprogramming of B cell precursors to induced pluripotent stem cells; C/EBPα facilitates transient chromatin accessibility and accelerates expression of pluripotency genes through a mechanism that involves activation of the Tet2 enzyme. A new study by Thomas Graf and colleagues describes how a pulse of C/EBPα (the transcription factor CCAAT/enhancer binding protein-α) followed by overexpression of the Yamanaka 'OSKM' reprogramming factors leads to fast and very efficient reprogramming of B-cell precursors to induced pluripotent stem (iPS) cells. The authors found that C/EBPα facilitates chromatin accessibility and accelerates expression of pluripotency genes through a mechanism that involves activation of the Tet2 enzyme. This demonstration of highly efficient and fast reprogramming of B cells into iPS cells provides a model for the study of the reprogramming process and may also have clinical relevance. CCAAT/enhancer binding protein-α (C/EBPα) induces transdifferentiation of B cells into macrophages at high efficiencies and enhances reprogramming into induced pluripotent stem (iPS) cells when co-expressed with the transcription factors Oct4 (Pou5f1), Sox2, Klf4 and Myc (hereafter called OSKM)1,2. However, how C/EBPα accomplishes these effects is unclear. Here we find that in mouse primary B cells transient C/EBPα expression followed by OSKM activation induces a 100-fold increase in iPS cell reprogramming efficiency, involving 95% of the population. During this conversion, pluripotency and epithelial–mesenchymal transition genes become markedly upregulated, and 60% of the cells express Oct4 within 2 days. C/EBPα acts as a ‘path-breaker’ as it transiently makes the chromatin of pluripotency genes more accessible to DNase I. C/EBPα also induces the expression of the dioxygenase Tet2 and promotes its translocation to the nucleus where it binds to regulatory regions of pluripotency genes that become demethylated after OSKM induction. In line with these findings, overexpression of Tet2 enhances OSKM-induced B-cell reprogramming. Because the enzyme is also required for efficient C/EBPα-induced immune cell conversion3, our data indicate that Tet2 provides a mechanistic link between iPS cell reprogramming and B-cell transdifferentiation. The rapid iPS reprogramming approach described here should help to fully elucidate the process and has potential clinical applications.

Published

2013

23. AllProbes_AllReplicates.xls

Author

Bruno Di Stefano, Samuel Collombet, Thomas Graf, Bruno Di Stefano, Samuel Collombet, and Thomas Graf

Published

2014

24. C/EBPα Activates Pre-existing and De Novo Macrophage Enhancers during Induced Pre-B Cell Transdifferentiation and Myelopoiesis

Author

Samuel Collombet, Miguel Beato, Aimee I. Badeaux, Guillermo P. Vicent, Yang Shi, Constanze Bonifer, Lars H. Bussmann, Jose Luis Sardina, Denis Thieffry, Maarten Hoogenkamp, Chris van Oevelen, Thomas Graf, and Cyrille Lepoivre

Subjects

Cell type, Cèl·lules B, Enhancer RNAs, Biology, Biochemistry, Article, Cell Line, CCAAT-Enhancer-Binding Protein-alpha, Genetics, medicine, Humans, Myeloid Cells, Enhancer, lcsh:QH301-705.5, B cell, Myelopoiesis, B-Lymphocytes, lcsh:R5-920, Proto-Oncogene Proteins c-ets, Cèl·lules mare embrionàries, Pioneer factor, Transdifferentiation, Cell Biology, Cell biology, medicine.anatomical_structure, lcsh:Biology (General), Cell Transdifferentiation, lcsh:Medicine (General), Developmental Biology

Abstract

Summary Transcription-factor-induced somatic cell conversions are highly relevant for both basic and clinical research yet their mechanism is not fully understood and it is unclear whether they reflect normal differentiation processes. Here we show that during pre-B-cell-to-macrophage transdifferentiation, C/EBPα binds to two types of myeloid enhancers in B cells: pre-existing enhancers that are bound by PU.1, providing a platform for incoming C/EBPα; and de novo enhancers that are targeted by C/EBPα, acting as a pioneer factor for subsequent binding by PU.1. The order of factor binding dictates the upregulation kinetics of nearby genes. Pre-existing enhancers are broadly active throughout the hematopoietic lineage tree, including B cells. In contrast, de novo enhancers are silent in most cell types except in myeloid cells where they become activated by C/EBP factors. Our data suggest that C/EBPα recapitulates physiological developmental processes by short-circuiting two macrophage enhancer pathways in pre-B cells., Graphical Abstract, Highlights • C/EBPα activates two classes of prospective myeloid enhancers in B cells • Pre-existing enhancers are bound by PU.1 and become hyper-activated by C/EBPα • C/EBPα acts as a pioneer factor with delayed kinetics on de novo enhancers • The two types of enhancers direct myeloid cell fate in B cells and hematopoiesis, In this study, Graf and colleagues show that, during B-cell-to-macrophage transdifferentiation, C/EBPα activates two types of myeloid enhancers in B cells. The two enhancer types are differentially activated, dictating gene expression levels of macrophage genes during the conversion of B cells into macrophages and normal hematopoiesis.