Structural and Functional Characterization of the MBD2-NuRD Co-Repressor Complex

Desai, Megha

01 January 2014

The MBD2-NuRD co-repressor complex is an epigenetic regulator of the developmental silencing of embryonic and fetal β-type globin genes in adult erythroid cells as well as aberrant methylation-dependent silencing of tumor suppressor genes in neoplastic diseases. Biochemical characterization of the MBD2-NuRD complex in chicken erythroid cells identified RbAp46/48, HDAC1/2, MTA1/2/3, p66α/β, Mi2α/β and MBD2 to comprise this multi-protein complex. In the work presented in Chapter 2, we have pursued biophysical and molecular studies to describe a previously uncharacterized domain of human MBD2 (MBD2IDR). Biophysical analyses show that MBD2IDR is an intrinsically disordered region (IDR). Despite this inherent disorder, MBD2IDR increases the overall binding affinity of MBD2 for methylated DNA. MBD2IDR also recruits the histone deacetylase core components (RbAp48, HDAC2 and MTA2) of NuRD through a critical area of contact requiring two contiguous amino acid residues, Arg286 and Leu287. Mutation of these critical residues abrogates interaction of MBD2 with the histone deacetylase core and impairs the ability of MBD2 to repress the methylated tumor suppressor gene Prostasin in MDA-MB-435 breast cancer cells. These findings expand our knowledge of the multi-dimensional interactions of the MBD2-NuRD complex that govern its function. In Chapter 3, we have discussed a novel mechanism for MBD2-mediated silencing of the fetal γ-globin gene. Through microarray expression analyses in adult erythroid cells of MBD2-/- mice, we identified ZBTB32 and miR-210 as downstream targets of MBD2. Over-expression of ZBTB32 and miR-210 in adult erythroid cells causes increased expression of the silenced fetal γ-globin gene. Thus, our results indicate that MBD2 may regulate γ-globin gene expression indirectly though ZBTB32 and miR-210 in adult erythroid cells.

MBD2

globin

epigenetics

tumor suppressor PRSS8

intrinsically disordered region

histone deacetylase

Genetics

Genomics

Molecular Biology

Molecular Genetics

Characterizing the role of Nucleosome Remodeling Factor (NURF) in tumorigenesis and metastatic progression using mouse models of breast cancer.

Alkhatib, Suehyb

20 June 2012

Increasingly the role of epigenetic machinery as a bridge between underlying DNA sequence and cellular phenotype is being discovered. The establishment of a myriad of unique cellular types sharing identical gene sequences in a multicellular organism gives a broad sense for the inherent role of epigenetic influence on cell differentiation. Importantly, the epigenetic mechanisms involved in establishing cell identity unsurprisingly contribute to diseased states, including cancer. Recent research continues to elucidate contributory roles of epigenetic mechanisms, such as DNA methylation, histone modification, and microRNA regulation, in human cancers. Additionally, chromatin remodelers, such as the Nucleosome Remodeling Factor (NURF), have been identified as important regulators for normal cell biology. While much has been done to identify and characterize the role of NURF chromatin remodeling complex as a key regulator of development in a number of model organisms, little has been published on the implications of NURF in diseases such as cancer. Our preliminary data shows dysregulation of E-cadherins, N-cadherins, and MHC-I genes in Bptf (an essential subunit of NURF) knocked down murine breast cancer cell lines. These proteins have well documented roles in the development and metastatic progression of cancers. To study the effect of Bptf knockdown on the development and progression of cancer we injected Bptf knocked down mouse breast cancer cell lines, 4T1, 66cl4, and 67NR, into syngenic BALB/c mice. Our findings reveal decreased tumor growth in 66cl4 and 67NR as measured by tumor weight at 3-4 weeks post injection. Tumor growth did not appear to be significantly affected in 4T1 challenged mice. However, mice inoculated with Bptf knockdown 4T1 cell lines have decreased metastasis to lungs as compared to control while metastasis of 66cl4 tumors to the lungs appear unaffected. To assess the role of the immune system in decreasing tumor growth in BALB/c mice, we injected 66cl4 tumors into NOD-SCID-Gamma (NSG) immune deficient mice. The tumors from these mice show no difference in tumor growth between Bptf knockdown and control tumors, implicating a role for the immune system regulating the decreased tumor weight in BALB/c mice. To delineate which immune cell effector may impede breast cancer carcinogenesis, we performed an in vitro natural killer (NK) cell cytotoxicity assay against 66cl4 tumors and found greater susceptibility to NK killing in Bptf knockdown tumors.

NURF

Nucleosome Remodeling Factor

Chromatin Remodeling

Breast Cancer

4T1

66cl4

Metastasis

Tumorigenesis

Mouse Model

Epigenetics

Immunoediting

Natural Killer

NK

Bptf

MDSC

Medical Genetics

Medical Sciences

Medicine and Health Sciences

Epigenetic approaches to the study of macrophages in atherosclerosis

Reschen, Michael

January 2015

Coronary artery disease (CAD) is caused by atherosclerosis, a chronic inflammatory response to modified lipoproteins. A key pathophysiological event is the lipid-induced transformation of macrophages into lipid-laden foam cells and their accumulation in atherosclerotic plaques. Heritable CAD risk is associated with common genetic variants at over 40 genomic loci; the underlying causal mechanisms remain largely unknown and could affect transcriptional regulation in foam cells. Epigenetic and gene expression changes were measured in primary human macrophages before and after exposure to atherogenic, oxidized low-density lipoprotein—with resultant foam cell formation. This unbiased approach involved open chromatin mapping with formaldehyde-assisted isolation of regulatory elements with enhancer and transcription factor mapping using chromatin immuno-precipitation. Foam cell formation was associated with changes in a subset of open chromatin and enhancer sites that were strongly correlated with expression of nearby genes. OxLDL-regulated enhancers were enriched for several transcription factors—including C/EBP-beta— that have no previously documented role in foam cell formation. OxLDL exposure up-regulated C/EBP-beta expression and increased C/EBP-beta binding across the genome, most prominently around genes involved in inflammatory response pathways. Variants at CAD-associated loci were enriched in the subset of oxLDLregulated open chromatin sites. These included rs72664324 in an oxLDL-induced super-enhancer at the PPAP2B locus. OxLDL increased C/EBP-beta binding at rs72664324. C/EBP-beta binding, enhancer activity and oxLDL-induced upregulation of PPAP2B were stronger with the protective A allele of rs72664324. The PPAP2B protein product LPP3 was expressed in foam cells in human atherosclerotic plaques and was upregulated by oxLDL exposure in macrophages, so increasing the degradation of pro-inflammatory mediators. I also found several other CAD risk candidate genes were regulated by oxLDL: Phosphatase and actin regulator 1 (PHACTR1) and macrophage inducible Ca²⁺ dependent C-type lectin (Mincle). This led us to find a novel expression-quantitative-trait locus for PHACTR1 in macrophages and define new glycolipid ligands for Mincle. Our results demonstrate a genetic mechanism contributing to CAD risk at the PPAP2B locus and highlight the value of integrating gene expression and epigenetic changes to study disease processes involving pathogenic environmental stimuli.

Dynamique de la variation génétique et épigénétique chez un vertébré kleptogène

Beauregard, France

01 1900

La variation phénotypique est essentielle à la persistance des organismes dans le temps ainsi qu’à la colonisation de nouveaux habitats. Les principales sources de variation phénotypique sont la génétique et l'épigénétique. L'épigénétique a été proposé comme un atout important pour les organismes asexués pour compenser le manque de diversité génétique. L'objectif de cette étude est d'évaluer si l’absence de variation génétique est compensée par l'épigénétique en comparant les profils de méthylation d’individus gynogènes et kleptogènes des hybrides de salamandre à points bleus. Les individus échantillonnés s’organisent en cinq groupes génétiquement différenciés, provenant du même haplome paternel A. jeffersonianum. Deux des cinq groupes sont exclusivement gynogènes, pour des raisons écologiques ou génomiques. Les trois autres groupes sont formés d’individus parfois kleptogènes, car ils présentent une variation génétique plus élevée au sein d’un site qu’entre les sites, en plus de porter des allèles très divergents par rapport à la distribution globale des allèles hybrides, trouvés en haute fréquence dans les populations sympatriques de A. laterale. Les patrons épigénétiques sont variables et distincts entre les cinq groupes génétiques. Les groupes gynogènes sont les seuls à présenter un effet environnemental significatif sur leurs patrons épigénétiques, suggérant que ces individus clonaux doivent être en mesure de maximiser leur potentiel de variation épigénétique pour faire face à des variations environnementales. / Phenotypic variation is critical to the persistence of organisms over time and the colonization of new habitats. The main consistent sources of phenotypic variation are genetics and epigenetics. Epigenetics was proposed as a valuable asset for asexual organisms to compensate or to complete genetic diversity. The objective of this study is to assess whether lack of genetic variation is compensated by epigenetics by comparing methylation patterns of gynogen and kleptogen individuals of the blue-spotted salamander hybrids. Individuals sampled clustered in five genetically differentiated groups, derived from the very same paternal A. jeffersonianum haplome. Two out of the five groups are exclusively gynogenetic, for either ecological or genomic factors. The other three groups occasionally formed kleptogen individuals, since they display a higher genetic variation within sites than among sites, in addition of displaying highly divergent alleles found in high frequency in the sympatric A. laterale populations. Epigenetic patterns are variable and distinct among the five genetic groups. Gynogenetic groups are the only one to display a significant environmental effect on their epigenetic pattern, suggesting clonal individuals must be able to make the most from their epigenetic variation potential to deal with environmental variations.

Épigénétique

Variation génétique

Kleptogénèse

Plasticité phénotypique

Unisexués

Ambystoma

Epigenetics

Genetic variation

Kleptogenesis

Unisexuals

Phenotypic plasticity

Funkční analýza genomu pomocí mapování integračních míst podporujících expresi retrovirů v lidských buňkách / Functional genome analysis using the retroviral integration sites permissive for provirus expression in human cells

Miklík, Dalibor

January 2013

The expression of retroviral genes depends on the establishment of the provirus - the DNA copy of retroviral genome integrated into the host genome. The transcriptional state of provirus is then influenced by the environment at the site of integration. The phenomenon of proviral silencing is an obstacle to the usage of retroviral vectors and a barrier to the eradication of human immunodeficiency virus type 1 (HIV-1) from infected individuals. Taking advantage of single cell clones bearing one provirus, this diploma thesis investigates the distribution of (epi)genomic features at the sites occupied by stably expressed proviruses. In total, long-term expression profiles of 245 and 255 clones carrying avian sarcoma-leucosis virus (ASLV) and HIV-1, respectively, were obtained. The database-based analysis of 42 integration sites of ASLV and three integration sites of HIV-1 proviruses shows that proviral stable expression highly correlates with the transcriptional start sites (TSS) at the sites of integration. Histone marks characteristic for the proximity of active TSSs and regulatory elements at the sites of integration of stably expressed proviruses confirm this finding. The results presented in this thesis could inspire other analyses investigating the relationship between the integration site and the...

Rôle de la protéine TRRAP, co-facteur des HATs, dans la régulation de la pluripotence des cellules souches embryonnaires et hématopoiétiques / TRRAP : an essential player in the regulation of stemness in embryonic and hematopoietic stem cells

Sawan-Vaissière, Carla

22 September 2010

Les cellules souches embryonnaires et adultes sont strictement contrôlées et régulées par différents mécanismes comme l’auto-renouvellement, la différentiation et l’apoptose. Les enzymes impliquées dans la modification des histones et les différents statuts de la chromatine seraient responsables de la mise en place, du maintien et de la propagation des différents profils d’expression des gènes mais le mécanisme sous-jacent reste néanmoins mal compris. Dans nos études, nous avons identifié le rôle de Trrap, un cofacteur des histones acétyltransférases dans le maintien de l’auto-renouvellement des cellules souches embryonnaires et adultes. La perte de la moelle épinière et une mortalité croissante sont survenues suite à la délétion conditionnelle du gène Trrap chez la souris. Ceci est dû à la perte des cellules hématopoïétiques progénitrices ainsi que des cellules hématopoïétiques souches par un mécanisme cellulaire autonome. L’analyse des cellules progénitrices, purifiées, de la moelle épinière à permis de révéler que ces anomalies sont associées à l’induction de l’apoptose indépendante de p53 ainsi qu’à la dérégulation des facteurs de transcription Myc. De plus, la délétion conditionnelle de Trrap dans les cellules souches embryonnaires induit la différentiation due au rôle important que Trrap joue dans la régulation du couplage de la méthylation de l’histone H3 aux lysines K4 et K27 appelées « domaines bivalents », le maintien du statut hyperdynamique de la chromatine et la régulation des gènes spécifiques à l’auto-renouvellement. Ceci est cohérent avec l’essentiel rôle de Trrap impliqué dans le mécanisme qui restreint l’induction de l’apoptose ou de la différentiation, ceci selon le type de cellules souches, et favorise le maintien de l’auto-renouvellement. Ces études ont permis d’identifier les différents rôles essentiels que Trrap joue dans le mécanisme qui permet le maintien des cellules souches embryonnaires et adultes ce qui soulève la possibilité que Trrap et les modifications des histones qui contrôlent l’auto-renouvellement pourraient être importants pour le développement et le maintien des cellules souches cancéreuses. Une meilleure compréhension du mécanisme commun qui implique Trrap et les modifications des histones contrôlant les éléments essentiels des cellules souches normales et cancéreuses s’avèrerait essentiel et très bénéfique pour les stratégies de thérapies épigénétiques qui ont pour but d’éradiquer les cellules souches cancéreuses / Embryonic and adult stem cells are tightly controlled and regulated by self-renewal, differentiation and apoptosis. Histone modifiers and chromatin states are believed to govern establishment, maintenance, and propagation of distinct patterns of gene expression in stem cells, however the underlying mechanism remains poorly understood. In our studies, we identified a role for the histone acetyltransferase cofactor Trrap in the maintenance of embryonic stem cells and hematopoietic stem/progenitor cells. Conditional deletion of the Trrap gene in mice resulted in ablation of bone marrow and increased lethality. This was due to the depletion of early hematopoietic progenitors, including hematopoietic stem cells, via a cell-autonomous mechanism. Analysis of purified bone marrow progenitors revealed that these defects are associated with induction of p53-independent apoptosis and deregulation of Myc transcription factors. Moreover, conditional deletion of Trrap in embryonic stem cells was found to results in unscheduled differentiation. This was due to the essential role of Trrap in coupling of H3K4 and H3K27 methylation ("bivalent-domains"), the maintenance of hyperdynamic chromatin state and regulation of the stemness genes, consistent with the essential function of Trrap in the mechanism that restricts apoptosis or differentiation depending on stem cell type and promotes the maintenance of self-renewal. Together, these studies have identified critical roles for Trrap in the mechanism that maintains embryonic and hematopoietic stem cells and raise the possibility that Trrap and histone modifications controlling self-renewal may be important for the development and maintenance of cancer stem cells. Better understanding of a common molecular mechanism involving HATs and histone modifications that controls key features of normal and cancer stem cells may prove highly beneficial for epigenetics-based therapeutic strategies aiming to eradicate cancer stem cells

TRRAP

Épigénétiques

Embryonnaire

Hématopoiétique

Cellules souches

Auto-renouvellement

Pluripotence

Différenciation

TRRAP

Epigenetics

Embryonic

Hematopoietic

Stem cell

Self-renewal

Pluripotency

Differenciation

571.6

DNA methylation : a hallmark of cancer mediating critical cellular processes in lung tumor / Méthylation de l'ADN : dispositif de traçage du cancer dans les processus cellulaires fondamentaux des tumeurs pulmonaires

Vaissière, Thomas

22 December 2010

Les mécanismes épigénétiques sont apparus comme fondamentaux au cours de la tumorigenèse, où l’inhibition des gènes suppresseurs de tumeurs et d'autres gènes associés aux cancers peut être causée non seulement par des facteurs génétiques, mais aussi épigénétiques. La réversibilité intrinsèque et l'ubiquité des modifications épigénétiques ainsi que leurs apparitions précoces dans de nombreux cancers en font une cible attractive pour la découverte de biomarqueurs et l’élaboration de stratégies pour la prévention du cancer. Afin d'identifier les événements épigénétiques impliqués dans la cancérogenèse et d’acquérir une meilleure compréhension des mécanismes, nous avons utilisé des méthodes quantitatives permettant de déterminer les profils de méthylation de l'ADN au sein d’un panel de gènes associés au cancer. Ces travaux ont principalement été effectués sur des cas de cancer du poumon et des contrôles. Nos analyses ont révélé une fréquence élevée et anormale d’hyperméthylation de l’ADN au niveau de gènes spécifiques dans les tumeurs pulmonaires par rapport aux tissus environnants non-tumoraux. Ces résultats sont en accord avec l'hypothèse établie qu’une méthylation aberrante de l'ADN se produit d’une manière tumeur-spécifiques et au niveau de certains gènes. Nous avons montré une association entre les changements de méthylation de l’ADN des gènes et certains facteurs environnementaux connus pour être des facteurs de risque (tels que le tabagisme et la consommation d’alcool). Nos résultats suggèrent également que les caractéristiques clinico-pathologiques tels que l'âge et le sexe peuvent influencer les niveaux de méthylation de l’ADN. Nous avons étudiés les conséquences moléculaires de l’inactivation des gènes ayant une hyperméthylation anormale dans les tumeurs et nous avons montré que leur dérégulation par voie épigénétique compromettait des voies de signalisation importantes (telles que les voies de signalisation déclenchant la mort cellulaire) / Epigenetic changes have emerged as key mechanisms in fpment. The main events associated with cancer development and progression such as silencing of tumor suppressor genes and activation of proto-oncogenes can be caused not only by genetic but also by epigenetic deregulation. The intrinsic reversibility and ubiquity of epigenetic changes as well as their early appearances in virtually all types of human cancer make them attractive subjects for biomarker discovery and strategies for cancer prevention. In order to identify critical epigenetic events involved in common human cancers and to gain a better mechanistic understanding of them we have applied quantitative profiling of DNA methylation states in a panel of cancer-associated genes in large case-control studies of lung cancer. Our analyses revealed a high frequency of aberrant hypermethylation of specific genes in lung tumors as compared to surrounding non-tumor tissues, consistent with the notion that aberrant DNA methylation occurs in a tumor-specific and gene-specific manner. Importantly, we have identified specific DNA methylation changes that are associated with the established and suspected risk factors (such as tobacco smoking and alcohol intake). Our results also indicated that clinicopathological features such as age and gender may also influence DNA methylation levels. Furthermore, we have carried out functional studies and identified possible underlying mechanisms and functional impact of deregulated methylation-mediated silencing of the genes under study on cellular processes (such as cell death response)

Méthylation de l’ADN

Épigénétiques

Tumorigénèse

Cancer du poumon

Réparation de l’ADN

Apoptose

Facteurs de risques

DNA methylation

Epigenetics

Tumorigenesis

Lung cancer

DNA repair

Apoptosis

Risk factors

572.8645

Studium epigenetických regulací HLA genů II. třídy v rámci příbuzenských vztahů. / The study of epigenetic regulation of gene HLA II. Clas within family relationships

Chmel, Martin

January 2015

Introduction: At our post-genomic era the studies of epigenetic regulation constitutes one of the tools for understanding the function of genes. Epigenetic regulation can directly control the temporal and spatial gene activity or silencing. The molecular basis of these regulations are DNA bases modifications, chromatin remodeling and RNA interference. At the same time, these mechanisms have a special way of transferring genetic information to subsequent generations called epigenetic inheritance. It has been proven epigenetic deregulation of certain genes as cause for many disease. For this reason, the study of epigenome HLA genes seems particularly important because these genes play a fundamental role in regulating the immune system. Aims: The aim of this work is to create a description of epigenetic modifications within families. It is an analysis of histone modifications and DNA methylation in the promoter region of the gene HLA DQA1. The aim was also to compare the differences in epigenetic modifications between alleles and compared the differences in these modifications between generations. The results will be compared with the analysis of the level of expression of the gene HLA DQA1. Methods: From collected peripheral blood of donors were isolated DNA, RNA, and leukocytes. DNA was used for...

The Eukaryotic Chromatin Computer

Arnold, Christian

01 November 2016

Eukaryotic genomes are typically organized as chromatin, the complex of DNA and proteins that forms chromosomes within the cell\\\'s nucleus. Chromatin has pivotal roles for a multitude of functions, most of which are carried out by a complex system of covalent chemical modifications of histone proteins. The propagation of patterns of these histone post-translational modifications across cell divisions is particularly important for maintenance of the cell state in general and the transcriptional program in particular. The discovery of epigenetic inheritance phenomena - mitotically and/or meiotically heritable changes in gene function resulting from changes in a chromosome without alterations in the DNA sequence - was remarkable because it disproved the assumption that information is passed to daughter cells exclusively through DNA. However, DNA replication constitutes a dramatic disruption of the chromatin state that effectively amounts to partial erasure of stored information. To preserve its epigenetic state the cell reconstructs (at least part of) the histone post-translational modifications by means of processes that are still very poorly understood. A plausible hypothesis is that the different combinations of reader and writer domains in histone-modifying enzymes implement local rewriting rules that are capable of \\\"recomputing\\\" the desired parental patterns of histone post-translational modifications on the basis of the partial information contained in that half of the nucleosomes that predate replication. It is becoming increasingly clear that both information processing and computation are omnipresent and of fundamental importance in many fields of the natural sciences and the cell in particular. The latter is exemplified by the increasingly popular research areas that focus on computing with DNA and membranes. Recent work suggests that during evolution, chromatin has been converted into a powerful cellular memory device capable of storing and processing large amounts of information. Eukaryotic chromatin may therefore also act as a cellular computational device capable of performing actual computations in a biological context. A recent theoretical study indeed demonstrated that even relatively simple models of chromatin computation are computationally universal and hence conceptually more powerful than gene regulatory networks. In the first part of this thesis, I establish a deeper understanding of the computational capacities and limits of chromatin, which have remained largely unexplored. I analyze selected biological building blocks of the chromatin computer and compare it to system components of general purpose computers, particularly focusing on memory and the logical and arithmetical operations. I argue that it has a massively parallel architecture, a set of read-write rules that operate non-deterministically on chromatin, the capability of self-modification, and more generally striking analogies to amorphous computing. I therefore propose a cellular automata-like 1-D string as its computational paradigm on which sets of local rewriting rules are applied asynchronously with time-dependent probabilities. Its mode of operation is therefore conceptually similar to well-known concepts from the complex systems theory. Furthermore, the chromatin computer provides volatile memory with a massive information content that can be exploited by the cell. I estimate that its memory size lies in the realms of several hundred megabytes of writable information per cell, a value that I compare with DNA itself and cis-regulatory modules. I furthermore show that it has the potential to not only perform computations in a biological context but also in a strict informatics sense. At least theoretically it may therefore be used to calculate any computable function or algorithm more generally. Chromatin is therefore another representative of the growing number of non-standard computing examples. As an example for a biological challenge that may be solved by the \\\"chromatin computer\\\", I formulate epigenetic inheritance as a computational problem and develop a flexible stochastic simulation system for the study of recomputation-based epigenetic inheritance of individual histone post-translational modifications. The implementation uses Gillespie\\\'s stochastic simulation algorithm for exactly simulating the time evolution of the chemical master equation of the underlying stochastic process. Furthermore, it is efficient enough to use an evolutionary algorithm to find a system of enzymes that can stably maintain a particular chromatin state across multiple cell divisions. I find that it is easy to evolve such a system of enzymes even without explicit boundary elements separating differentially modified chromatin domains. However, the success of this task depends on several previously unanticipated factors such as the length of the initial state, the specific pattern that should be maintained, the time between replications, and various chemical parameters. All these factors also influence the accumulation of errors in the wake of cell divisions. Chromatin-regulatory processes and epigenetic (inheritance) mechanisms constitute an intricate and sensitive system, and any misregulation may contribute significantly to various diseases such as Alzheimer\\\'s disease. Intriguingly, the role of epigenetics and chromatin-based processes as well as non-coding RNAs in the etiology of Alzheimer\\\'s disease is increasingly being recognized. In the second part of this thesis, I explicitly and systematically address the two hypotheses that (i) a dysregulated chromatin computer plays important roles in Alzheimer\\\'s disease and (ii) Alzheimer\\\'s disease may be considered as an evolutionarily young disease. In summary, I found support for both hypotheses although for hypothesis 1, it is very difficult to establish causalities due to the complexity of the disease. However, I identify numerous chromatin-associated, differentially expressed loci for histone proteins, chromatin-modifying enzymes or integral parts thereof, non-coding RNAs with guiding functions for chromatin-modifying complexes, and proteins that directly or indirectly influence epigenetic stability (e.g., by altering cell cycle regulation and therefore potentially also the stability of epigenetic states). %Notably, we generally observed enrichment of probes located in non-coding regions, particularly antisense to known annotations (e.g., introns). For the identification of differentially expressed loci in Alzheimer\\\'s disease, I use a custom expression microarray that was constructed with a novel bioinformatics pipeline. Despite the emergence of more advanced high-throughput methods such as RNA-seq, microarrays still offer some advantages and will remain a useful and accurate tool for transcriptome profiling and expression studies. However, it is non-trivial to establish an appropriate probe design strategy for custom expression microarrays because alternative splicing and transcription from non-coding regions are much more pervasive than previously appreciated. To obtain an accurate and complete expression atlas of genomic loci of interest in the post-ENCODE era, this additional transcriptional complexity must be considered during microarray design and requires well-considered probe design strategies that are often neglected. This encompasses, for example, adequate preparation of a set of target sequences and accurate estimation of probe specificity. With the help of this pipeline, two custom-tailored microarrays have been constructed that include a comprehensive collection of non-coding RNAs. Additionally, a user-friendly web server has been set up that makes the developed pipeline publicly available for other researchers. / Eukaryotische Genome sind typischerweise in Form von Chromatin organisiert, dem Komplex aus DNA und Proteinen, aus dem die Chromosomen im Zellkern bestehen. Chromatin hat lebenswichtige Funktionen in einer Vielzahl von Prozessen, von denen die meisten durch ein komplexes System von kovalenten Modifikationen an Histon-Proteinen ablaufen. Muster dieser Modifikationen sind wichtige Informationsträger, deren Weitergabe über die Zellteilung hinaus an beide Tochterzellen besonders wichtig für die Aufrechterhaltung des Zellzustandes im Allgemeinen und des Transkriptionsprogrammes im Speziellen ist. Die Entdeckung von epigenetischen Vererbungsphänomenen - mitotisch und/oder meiotisch vererbbare Veränderungen von Genfunktionen, hervorgerufen durch Veränderungen an Chromosomen, die nicht auf Modifikationen der DNA-Sequenz zurückzuführen sind - war bemerkenswert, weil es die Hypothese widerlegt hat, dass Informationen an Tochterzellen ausschließlich durch DNA übertragen werden. Die Replikation der DNA erzeugt eine dramatische Störung des Chromatinzustandes, welche letztendlich ein partielles Löschen der gespeicherten Informationen zur Folge hat. Um den epigenetischen Zustand zu erhalten, muss die Zelle Teile der parentalen Muster der Histonmodifikationen durch Prozesse rekonstruieren, die noch immer sehr wenig verstanden sind. Eine plausible Hypothese postuliert, dass die verschiedenen Kombinationen der Lese- und Schreibdomänen innerhalb von Histon-modifizierenden Enzymen lokale Umschreibregeln implementieren, die letztendlich das parentale Modifikationsmuster der Histone neu errechnen. Dies geschieht auf Basis der partiellen Informationen, die in der Hälfte der vererbten Histone gespeichert sind. Es wird zunehmend klarer, dass sowohl Informationsverarbeitung als auch computerähnliche Berechnungen omnipräsent und in vielen Bereichen der Naturwissenschaften von fundamentaler Bedeutung sind, insbesondere in der Zelle. Dies wird exemplarisch durch die zunehmend populärer werdenden Forschungsbereiche belegt, die sich auf computerähnliche Berechnungen mithilfe von DNA und Membranen konzentrieren. Jüngste Forschungen suggerieren, dass sich Chromatin während der Evolution in eine mächtige zelluläre Speichereinheit entwickelt hat und in der Lage ist, eine große Menge an Informationen zu speichern und zu prozessieren. Eukaryotisches Chromatin könnte also als ein zellulärer Computer agieren, der in der Lage ist, computerähnliche Berechnungen in einem biologischen Kontext auszuführen. Eine theoretische Studie hat kürzlich demonstriert, dass bereits relativ simple Modelle eines Chromatincomputers berechnungsuniversell und damit mächtiger als reine genregulatorische Netzwerke sind. Im ersten Teil meiner Dissertation stelle ich ein tieferes Verständnis des Leistungsvermögens und der Beschränkungen des Chromatincomputers her, welche bisher größtenteils unerforscht waren. Ich analysiere ausgewählte Grundbestandteile des Chromatincomputers und vergleiche sie mit den Komponenten eines klassischen Computers, mit besonderem Fokus auf Speicher sowie logische und arithmetische Operationen. Ich argumentiere, dass Chromatin eine massiv parallele Architektur, eine Menge von Lese-Schreib-Regeln, die nicht-deterministisch auf Chromatin operieren, die Fähigkeit zur Selbstmodifikation, und allgemeine verblüffende Ähnlichkeiten mit amorphen Berechnungsmodellen besitzt. Ich schlage deswegen eine Zellularautomaten-ähnliche eindimensionale Kette als Berechnungsparadigma vor, auf dem lokale Lese-Schreib-Regeln auf asynchrone Weise mit zeitabhängigen Wahrscheinlichkeiten ausgeführt werden. Seine Wirkungsweise ist demzufolge konzeptionell ähnlich zu den wohlbekannten Theorien von komplexen Systemen. Zudem hat der Chromatincomputer volatilen Speicher mit einem massiven Informationsgehalt, der von der Zelle benutzt werden kann. Ich schätze ab, dass die Speicherkapazität im Bereich von mehreren Hundert Megabytes von schreibbarer Information pro Zelle liegt, was ich zudem mit DNA und cis-regulatorischen Modulen vergleiche. Ich zeige weiterhin, dass ein Chromatincomputer nicht nur Berechnungen in einem biologischen Kontext ausführen kann, sondern auch in einem strikt informatischen Sinn. Zumindest theoretisch kann er deswegen für jede berechenbare Funktion benutzt werden. Chromatin ist demzufolge ein weiteres Beispiel für die steigende Anzahl von unkonventionellen Berechnungsmodellen. Als Beispiel für eine biologische Herausforderung, die vom Chromatincomputer gelöst werden kann, formuliere ich die epigenetische Vererbung als rechnergestütztes Problem. Ich entwickle ein flexibles Simulationssystem zur Untersuchung der epigenetische Vererbung von individuellen Histonmodifikationen, welches auf der Neuberechnung der partiell verlorengegangenen Informationen der Histonmodifikationen beruht. Die Implementierung benutzt Gillespies stochastischen Simulationsalgorithmus, um die chemische Mastergleichung der zugrundeliegenden stochastischen Prozesse über die Zeit auf exakte Art und Weise zu modellieren. Der Algorithmus ist zudem effizient genug, um in einen evolutionären Algorithmus eingebettet zu werden. Diese Kombination erlaubt es ein System von Enzymen zu finden, dass einen bestimmten Chromatinstatus über mehrere Zellteilungen hinweg stabil vererben kann. Dabei habe ich festgestellt, dass es relativ einfach ist, ein solches System von Enzymen zu evolvieren, auch ohne explizite Einbindung von Randelementen zur Separierung differentiell modifizierter Chromatindomänen. Dennoch ängt der Erfolg dieser Aufgabe von mehreren bisher unbeachteten Faktoren ab, wie zum Beispiel der Länge der Domäne, dem bestimmten zu vererbenden Muster, der Zeit zwischen Replikationen sowie verschiedenen chemischen Parametern. Alle diese Faktoren beeinflussen die Anhäufung von Fehlern als Folge von Zellteilungen. Chromatin-regulatorische Prozesse und epigenetische Vererbungsmechanismen stellen ein komplexes und sensitives System dar und jede Fehlregulation kann bedeutend zu verschiedenen Krankheiten, wie zum Beispiel der Alzheimerschen Krankheit, beitragen. In der Ätiologie der Alzheimerschen Krankheit wird die Bedeutung von epigenetischen und Chromatin-basierten Prozessen sowie nicht-kodierenden RNAs zunehmend erkannt. Im zweiten Teil der Dissertation adressiere ich explizit und auf systematische Art und Weise die zwei Hypothesen, dass (i) ein fehlregulierter Chromatincomputer eine wichtige Rolle in der Alzheimerschen Krankheit spielt und (ii) die Alzheimersche Krankheit eine evolutionär junge Krankheit darstellt. Zusammenfassend finde ich Belege für beide Hypothesen, obwohl es für erstere schwierig ist, aufgrund der Komplexität der Krankheit Kausalitäten zu etablieren. Dennoch identifiziere ich zahlreiche differentiell exprimierte, Chromatin-assoziierte Bereiche, wie zum Beispiel Histone, Chromatin-modifizierende Enzyme oder deren integrale Bestandteile, nicht-kodierende RNAs mit Führungsfunktionen für Chromatin-modifizierende Komplexe oder Proteine, die direkt oder indirekt epigenetische Stabilität durch veränderte Zellzyklus-Regulation beeinflussen. Zur Identifikation von differentiell exprimierten Bereichen in der Alzheimerschen Krankheit benutze ich einen maßgeschneiderten Expressions-Microarray, der mit Hilfe einer neuartigen Bioinformatik-Pipeline erstellt wurde. Trotz des Aufkommens von weiter fortgeschrittenen Hochdurchsatzmethoden, wie zum Beispiel RNA-seq, haben Microarrays immer noch einige Vorteile und werden ein nützliches und akkurates Werkzeug für Expressionsstudien und Transkriptom-Profiling bleiben. Es ist jedoch nicht trivial eine geeignete Strategie für das Sondendesign von maßgeschneiderten Expressions-Microarrays zu finden, weil alternatives Spleißen und Transkription von nicht-kodierenden Bereichen viel verbreiteter sind als ursprünglich angenommen. Um ein akkurates und vollständiges Bild der Expression von genomischen Bereichen in der Zeit nach dem ENCODE-Projekt zu bekommen, muss diese zusätzliche transkriptionelle Komplexität schon während des Designs eines Microarrays berücksichtigt werden und erfordert daher wohlüberlegte und oft ignorierte Strategien für das Sondendesign. Dies umfasst zum Beispiel eine adäquate Vorbereitung der Zielsequenzen und eine genaue Abschätzung der Sondenspezifität. Mit Hilfe der Pipeline wurden zwei maßgeschneiderte Expressions-Microarrays produziert, die beide eine umfangreiche Sammlung von nicht-kodierenden RNAs beinhalten. Zusätzlich wurde ein nutzerfreundlicher Webserver programmiert, der die entwickelte Pipeline für jeden öffentlich zur Verfügung stellt.

Histon-Modifikation

Epigenetik

Chromatin

biologischer Computer

Alzheimer

Gillespie

stochastische Simulation

histone modification

epigenetics

chromatin

biological computer

Alzheimer

Gillespie

stochastic simulation

ddc:000

The Chromatin Remodeler and Tumor Suppress Chd5 Promotes Expression and Processing of Transcripts During Development of the Zebrafish Neural System

Erin L Sorlien (6635906)

14 May 2019

<div>Vertebrate neurogenesis is a multistep process that coordinates complex signaling pathways and chromatin-based regulatory machinery to generate highly specialized cells (Hsieh and Zhao 2016; Urban and Guillemot 2014; Alunni and Bally-Cuif 2016; Yao and Jin 2014; Schmidt, Strahle, and Scholpp 2013). Epigenetic factors play a fundamental role in underwriting neurogenesis in part by contributing to control of gene expression in differentiating neurons. A mechanistic understanding of the epigenetic machinery underlying neurogenesis in vertebrates is necessary both to fully understand biogenesis of neural tissue in this subphylum as well as to develop effective therapeutic strategies to treat diseased or damaged neural tissue. </div><div>An example of an epigenetic factor that is important for both neuronal differentiation and disease states is CHD5, a vertebrate-specific member of the CHD family of ATP-dependent chromatin remodeling proteins. Chromodomain / Helicase / DNA-binding (CHD) proteins play a variety of roles in vertebrate development, and misregulation or loss of CHD proteins has been linked to numerous diseases (Mayes et al. 2014; Marfella and Imbalzano 2007; Bartholomew 2014). CHD5 is expressed primarily in neural tissue, where it is thought to contribute to neurogenesis, and has been strongly linked to tumor suppression (Thompson et al. 2003; Vestin and Mills 2013). Loss of CHD5 plays a significant role in development of neuroblastoma, a devastating tumor that is a leading cause of cancer-related death in children (Jiang, Stanke, and Lahti 2011; Maris and Matthay 1999). Consistent with the disease phenotype associated with loss of CHD5, reduced expression of CHD5 impairs differentiation of neuronal cells (Egan et al. 2013b). However, ablation of CHD5 in mice surprisingly resulted in no detectable defects in brain development (Li et al. 2014; Zhuang et al. 2014). A subsequent report revealed that mice conditionally ablated for CHD5 in neural tissue exhibit symptoms consistent with an autism spectrum disorder (Pisansky et al. 2017). Much remains to be learned about the role of CHD5 in these processes to clarify these observations.</div><div>Further, Chd5 is unique among the family of Chd remodelers in that it provides a biochemical basis for crosstalk between the critical epigenetic marks H3K27me3 and DNA methylation. Chd5 and the closely related remodelers Chd3 and Chd4 are all components of the Mi-2/NuRD histone deacetylase complex that plays a critical role in mediating transcriptional repression in response to DNA methylation in mammals (Allen, Wade, and Kutateladze 2013). Only CHD5 is preferentially expressed in neural tissue, however, and only Chd5 remodelers have biochemical evidence of direct interaction with H3K27me3, which plays a critical role in enabling proper expression of transcriptional programs during neurogenesis (Egan et al. 2013b). Chd5 is thus unique among CHD remodelers in that it is biochemically linked to both DNA methylation and H3K27me3 in addition to being preferentially expressed in neural tissue.</div><div>With regards to mechanism, much remains to be learned regarding how Chd5 remodelers contribute to gene expression and tumor suppression. However, the data to date do not show extensive transcript phenotypes and it is not clear how the biochemical action of CHD5 contributes to the neurological phenotypes ascribed to altered expression of CHD5. Therefore, it is critical to determine a suitable context to study the role of CHD5 in these processes. Identification of CHD5-dependent genes in neurons is likely to generate insight into how loss of CHD5 contributes to tumorigenesis, in particular with regards to development of neuroblastoma. Regulatory pathways that drive neurogenesis have been found to be extensively conserved between humans and zebrafish. Therefore, we have turned to the power of the zebrafish model system to characterize how loss of Chd5 alters brain development during embryogenesis.</div><div>Importantly zebrafish development, and neurogenesis in particular, occurs largely over the first 5-days of development. Zebrafish are born outside of the mother, which can produce large clutches of several hundred embryos per week, providing us with an accessible context to study the role of chd5, the zebrafish homolog of human CHD5. The central nervous system of the zebrafish develops rapidly, and shares many of the organization features of the mammalian brain (Kalueff, Stewart, and Gerlai 2014). In particular, neuroblastoma arises from a population of cells known as sympathetic ganglion cells that are derived from the neural crest (Pei et al. 2013). These cells are conserved in vertebrates, and several models to study how these cells transform into neuroblastoma exist in zebrafish (Zhu et al. 2017; Morrison et al. 2016; Zhu and Thomas Look 2016). However, our understanding of the mechanisms controlling ganglion cell differentiation is incomplete and requires further investigation to understand how epigenetic and transcriptional mechanisms contribute to development of these cells and how failure of these processes leads to cancer. The neural crest undergoes a series of differentiation steps to form mature sympathetic neurons that are guided by bone morphogenic protein signaling, and transcription changes (Ernsberger and Rohrer 2018). These cells express key enzymes for synthesizing dopamine and norephinephrine to control the sympathetic system throughout the central nervous system (Ernsberger and Rohrer 2018).</div><div>To address these questions about Chd5, we have used CRISPR/Cas9 to generate chd5-/- zebrafish that are protein nulls as determined by western blot. These chd5-/- fish are phenotypically indistinguishable from wild-type fish under standard growth conditions as was previously observed for mice lacking CHD5 (Zhuang et al. 2014; Li et al. 2014). By using zebrafish, we are able to perform transcriptome analyses to identify Chd5 target genes at stages much earlier than has previously been performed in mice because we can harvest large amounts of the tissue of interest from the readily accessible embryos. We have therefore undertaken RNA-seq analysis of isolated brains from wild-type and chd5-/- fish to identify chd5-dependent genes in predominantly differentiating (2-day old) and substantially differentiated (5-day old) neural tissue. These data provide a substantively different perspective from previous studies that examine the role of CHD5 in gene expression of differentiated SY-SH5Y cells (Egan et al. 2013a) or in the forebrain of 8-week-old mice (Pisansky et al. 2017). (Jiang, Stanke, and Lahti 2011). One role we identified from this data, is the promotion of development of sympathetic ganglion cells (detailed below), illuminating for the first time a role for chd5 in promoting differentiation of cells directly involved in neuroblatoma.</div><div>We observe not only extensive changes in gene expression, but also identify a novel role for Chd5 in enabling proper splicing during this critical window of neurogenesis in the zebrafish brain. We are further exploring the role of CHD5 in these processes by creating comparable cell culture-based models of loss of CHD5 to determine the conservation of molecular phenotypes observed in zebrafish. Furthermore, this model enables us to leverage the extensive biochemical tools available in cell culture to examine alterations to the chromatin that are difficult to interpret from studies of complex tissues such as the brain. </div><div>Herein I will describe the research progress we have made to understand the role of Chd5 in gene expression and splicing in zebrafish, as well as ongoing work to engineer mouse embryonic stem cells as an additional model to study the transcriptional consequences of loss of CHD5. Critically, the addition of the cell culture model will greatly enable biochemical characterization of the changes that are leading in particular to the changes in gene expression and splicing and will provide us with a context to test for a direct role of CHD5 in these processes. In addition, this thesis will detail the results from ongoing projects using the zebrafish model system, including: development of models in zebrafish to study the tumor suppressive role of Chd5, phenotypes observed using a targeted chemical-genetic screen, and advancement in developing new tools in zebrafish to engineer specific genomic modifications that will greatly expand the power of this vertebrate model.</div><div><br></div>

Cancer

Bioinformatics

CHD5

chromatin remodeling

neurogenesis

zebrafish

gene expression

alternative splicing

sympathetic ganglion cells

neuroblastoma