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Computational Study of Nucleosome Positioning Sequence Patterns and the Effects of the Nucleosome Positioning on the Availability of the Transcription Factor Binding Sites in Study SystemsYang, Doo Seok January 2017 (has links)
Nucleosomes, the primary unit of chromatin structure, are positioned either statistically or specifically. The statistical positioning denotes the arbitrary positioning of nucleosomes on DNA agreeing with the nucleosome’s broad coverage of the genome—however, there is evidence that nucleosomes are also positioned specifically at controlled positions. DNA sequences determine the specific nucleosome positions, and the presence or depletion of nucleosomes affects the availability of the DNA region to other proteins. The DNA sequences of H2A and H2A.Z nucleosomes in Drosophila were analysed in search of nucleosome positioning patterns. Dinucleotide patterns with 10 bp periodicity were identified from the DNA sequences of H2A nucleosomes. Compared with the yeast patterns, the Drosophila patterns had the same periodicity but different dinucleotides near the dyad, which was related to the different H3 structure between them. The nucleosome positioning patterns from the H2A.Z nucleosomes implied the specific histone-DNA interaction as a result of the deviations of the patterns where the different amino acids of H2A and H2A.Z interact with the DNA. The Ly49 gene cluster was selected as a model system to study the interplay between nucleosomes and transcription factors. Ly49 proteins, the surface receptors on NK cells, display variegated expression patterns, and the bidirectional promoter Pro-1 is known as a key determinant of the stochastic expression of each Ly49 gene. The systematic analysis of nucleosome positions based on the genome sequences in the Ly49 gene cluster revealed that the repressing Pro-1 reverse promoters are open, while the activating forward Pro-1 promoters were covered by nucleosomes. Furthermore, specific nucleosome positions covered transcription factor binding sites. The covered factor binding sites were further examined by their periodic appearances on the nucleosome-covered sequences, which revealed the accessibility to the sites. The sequence analysis predicted that the regulation by the transcription factor AML-1 would be sensitive to the nucleosome coverage; the prediction was confirmed by cell line experiments. The 10 bp periodic nucleosome positioning patterns interact with histones specifically. The long nucleosome positioning patterns coexist with the short sequence motifs for transcription factor binding sites adding another layer of the control to the transcriptional regulation.
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The role of H2A-H2B dimers in the mechanical stability of nucleosomesLuzzietti, Nicholas 29 November 2013 (has links)
Eukaryotic genomes are densely compacted into chromatin, so that they can be contained in the nucleus. Despite the tight packaging genes need to be accessible for normal metabolic activities to occur, such as transcription, repair and replication. These processes are regulated by a vast number of proteins but also by the level of compaction of chromatin. The translocation of motor proteins along DNA produces torsional stress which in turn alters chromatin compaction both upstream and downstream. Few single-molecule studies have investigated the behaviour of nucleosomes when subjected to torsion. The inability to measure the applied torque though represented a major limitation to those reports.
The implementation of the rotor bead assay, which allows to directly measure the torque applied in magnetic tweezers experiments, has been hindered by a difficult sample preparation procedure. In order to overcome this limitation an efficient protocol for the insertion of chemical or structural modifications in long DNA substrates was developed. This was then further expanded to allow the introduction of labels in multiple loci and/or both strands and has been used successfully in a number of studies.
Furthermore this is the first report of tensile experiments performed on nucleosomes with a histone variant. H2AvD nucleosomes were studied due to the interest in the biological role of H2A.Z-family proteins. Interestingly, the variant nucleosomes appear to bind less DNA and to be evicted from the DNA at lower forces than those observed for canonical nucleosomes. These findings show an important role for the H2A-H2B dimers in the mechanical stability of nucleosomes. Furthermore these results are in agreement with recently proposed models of a dynamic nucleosome, in contrast to the long-standing view of nucleosomes as static structures.:Abstract
Table of contents
1 Introduction
1.1 The transforming principle
1.2 Chromatin
1.2.1 Nucleosomes
1.2.2 The 30 nm fibre: a mirage?
1.2.3 Histone code
1.3 Histone variant H2A.Z
1.3.1 H2A.Z and transcription
1.4 Single molecule studies of chromatin
1.4.1 Chromatin under tension
1.4.2 Open nucleosome
1.4.3 Twisted chromatin
1.5 Single molecule techniques
1.5.1 Atomic force microscopy
1.5.2 Foerster resonance energy transfer
1.5.3 Magnetic tweezers
1.5.4 Worm-like chain model
2 Aims of the project
3 Cut and paste method for internal DNA labelling
3.1 Introduction
3.2 Experimental design
3.3 Results
3.3.1 Sequence design and cloning
3.3.2 Labelling and religation efficiency
3.3.3 Structural modifications
3.3.4 Labelling of multiple loci
3.3.5 Opposite-strand labelling
3.4 Discussion
4 Reconstituting chromatin
4.1 Long array of NPSs
4.1.1 Polymer physics applied to molecular cloning
4.1.2 Preventing homologous recombination
4.2 Expression and purification of histone proteins
4.2.1 Protein expression
4.2.2 Inclusions bodies
4.2.3 Histone purification
4.2.4 Octamer reconstitution and isolation
4.2.5 H2AvD
4.3 Reconstitution of nucleosomal arrays and biochemical analysis
4.3.1 Reconstitution procedure
4.3.2 Biochemical analysis
4.4 Tweezers construct with nucleosomes
5 Eviction of nucleosomes
5.1 Nucleosome eviction
5.1.1 A two-stage process
5.1.2 Chromatin fibres
5.1.3 Reassembly of nucleosomes
5.1.4 Distinct populations within nucleosome eviction events
5.1.5 Nicked and supercoilable nucleosomal arrays
5.2 Eviction of H2AvD-nucleosomes
5.2.1 H2AvD-nucleosomes bind less inner turn DNA
5.2.2 H2AvD-nucleosomes evict at lower forces
5.2.3 Likelihood of nucleosome reassembly
5.2.4 Gradual weakening of nucleosomes
5.2.5 Analysis software NucleoStep
5.3 Towards a rotor-bead assay on chromatin
5.4 Discussion
5.4.1 Nucleosome eviction in two stages
5.4.2 The fate of dimers in single molecule experiments
5.4.3 Structural origin and biological relevance of the mechanical properties
of H2AvD-nucleosomal core particles
5.4.4 Monolithic or dynamic nucleosomes
6 Conclusions
Bibliography
Appendix
6.1 Internal labelling Procedure
6.1.1 Cloning
6.1.2 Nicking & cutting
6.1.3 The replace reaction
6.1.4 Purification
6.1.5 Ligation (optional)
6.1.6 Opposite strand labelling
6.1.7 Assessing the results of the labelling reaction
6.2 Chromatin reconstitution
6.2.1 Long array of NPSs
6.2.2 Expression and purification of histone proteins
6.2.3 Reconstitution of nucleosomal arrays and biochemical characterization
6.2.4 Simple Phenol:chloroform isolation of DNA
6.3 Magnetic tweezers experiments
6.3.1 Flow cell assembly
6.3.2 Functionalization of flow cells
6.3.3 Magnetic tweezers and rotor bead measurements
6.3.4 Force calibration
List of Figures
List of Tables
List of publications
Acknowledgements
Declaration of originality
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Transcriptional Homeostasis and Chromatin DynamicsBryll, Alysia 13 April 2022 (has links)
Multiple regulatory mechanisms work to ensure that eukaryotic transcription maintains mRNA pools and subsequent protein synthesis. When errors in transcription occur, deleterious effects on cellular fitness can develop. RNA degradation as well as histone modifications, specifically at promoter proximal nucleosomes, play a critical role in maintaining transcription, but, exact mechanisms are not fully understood. In this dissertation, I investigate the role of RNA degradation and chromatin dynamics in transcription regulation as well as further understand, through biochemical analysis, a critical histone deacetylase.
Using various genome-wide methodologies in Saccharomyces cerevisiae, we find a functional interaction between the nuclear RNA exosome and histone variant H2A.Z that maintains mRNA levels. There is a reduction in RNA polymerase II nascent transcription following RNA exosome subunit Rrp6 depletion that is further globally accentuated with H2A.Z deposition loss. To understand the mechanism leading to this global reduction, we identify the mRNA of Sirtuin histone deacetylase Hst3 as a target of the RNA exosome, revealing a means to link degradation to the transcription machinery. These findings show that even slight changes in deacetylase or acetylase activity can have significant effects on transcription. Additionally, we reveal a global impact of H2A.Z on transcription.
We further investigate the functional and structural significance of human surtuin histone deacetylase SIRT6 (yeast homolog Hst3). Using histone deacetylase assays, we confirm the significance of specific residues of SIRT6 in nucleosome binding and deacetylase activity. Additionally, we show SIRT6 has reduced deacetylase activity in vitro on acetylated lysine 56 as compared to acetylated lysine 9 on histone H3. Finally, we confirm structural findings that the histone tail of H2A impacts SIRT6 H3K9Ac deacetylation activity.
Together, these findings indicate a critical importance of histone deacetylase activity in maintaining transcription, a novel role of H2A.Z in global transcription regulation that furthers our understanding of SIRT6 structure and function.
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A role for prefoldin in H2A.Z deposition in ArabidopsisMarí Carmona, Cristina 27 May 2021 (has links)
[ES] El complejo prefoldina (PFDc) participa en la proteostasis celular en eucariotas actuando como cochaperona de la chaperonina CTT. Este papel se ejerce principalmente en el citoplasma, donde contribuye al correcto plegamiento de las proteínas cliente, evitando así que se formen agregaciones y daño celular. Varios informes indican, sin embargo, que también juegan un papel en la regulación transcripcional en el núcleo en varias especies modelo. En este trabajo, hemos investigado cuán extendido es el papel de la PFD en los procesos nucleares al estudiar su interactoma y sus redes de coexpresión en levaduras, moscas y humanos. El análisis indica que pueden realizar una amplia y conservada variedad de funciones en procesos nucleares. La construcción del interactoma predicho para las PFD de Arabidopsis, basado en interacciones ortólogas, nos ha permitido identificar muchos putativos interactores de PFD que los vinculan a procesos no esperados, como la remodelación de la cromatina. Basados en este análisis, hemos investigado el papel de la PFD en la deposición de H2A.Z a través de su interacción con el complejo remodelador de la cromatina SWR1c. Nuestros resultados muestran que la PFD tienen un efecto positivo sobre SWR1c, lo que se refleja en defectos en la deposición de H2A.Z en cientos de genes en plántulas defectuosas en las actividades de PFD3 y PFD5. / [CA] El complex prefoldina (PFDc) participa a la proteostasis cel·lular en eucariotes actuant com co-xaperona de la xaperonina CTT. Aquest paper s'exerceix principalment en el citoplasma, on contribueix al correcte plegament de les proteïnes client, evitant així que es formen agregacions i dany cel·lular. Diversos informes indiquen, però, que també juguen un paper en la regulació transcripcional en el nucli en diverses espècies model. En aquest treball, hem investigat com d'estès és el paper de la PFD en els processos nuclears estudiant el seu interactoma i les seues xarxes de coexpressió en llevats, mosques i humans. L'anàlisi indica que poden realitzar una àmplia i conservada varietat de funcions en processos nuclears. La construcció de l'interactoma predit per a les PFD d'Arabidopsis, basat en interaccions ortòlegs, ens ha permès identificar molts interactors putatius de les PFDs que les vinculen a processos no esperats, com és la remodelació de la cromatina. Amb base en aquest anàlisi, hem investigat el paper de la PFD en la deposició d'H2A.Z a través de la seva interacció amb el complex remodelador de la cromatina SWR1c. Els nostres resultats mostren que les PFDs tenen un efecte positiu sobre SWR1c, que es reflecteix en defectes en la deposició de H2A.Z en centenars de gens en plàntules defectuoses en les activitats de PFD3 i PFD5 / [EN] The prefoldin complex (PFDc) participates in cellular proteostasis in eukaryotes by acting as cochaperone of the chaperonin CTT. This role is mainly exerted in the cytoplasm where it contributes to the correct folding of client proteins, thus preventing them to form aggregations and cellular damage. Several reports indicate, however, that they also play a role in transcriptional regulation in the nucleus in several model species. In this work, we have investigated how extended is the role of PFDs in nuclear processes by inspecting their interactome and their coexpression networks in yeast, fly, and humans. The analysis indicates that they may perform extensive, conserved functions in nuclear processes. The construction of the predicted interactome for Arabidopsis PFDs, based on the ortholog interactions, has allowed us to identify many putative PFD interactors linking them to unanticipated processes, such as chromatin remodeling. Based on this analysis, we have investigated the role of PFDs in H2A.Z deposition through their interaction with the chromatin remodeling complex SWR1c. Our results show that PFDs have a positive effect on SWR1c, which is reflected in defects in H2A.Z deposition in hundreds of genes in seedlings defective in PFD3 and PFD5 activities. / Esta Tesis doctoral ha sido posible gracias al contrato de formación de personal investigador ofrecido por la Universidad Politécnica de Valencia y a la financiación de Pedro J. Marí & Asociados. El proyecto al que pertenece este trabajo ha sido financiado por la Agencia Española de Investigación BIO2013-43184-P y BIO2016-79133-P / Marí Carmona, C. (2021). A role for prefoldin in H2A.Z deposition in Arabidopsis [Tesis doctoral]. Universitat Politècnica de València. https://doi.org/10.4995/Thesis/10251/167014
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Étude de la variante d’histone H2A.Z et du cycle de phosphorylation de l’ARN polymérase II chez Saccharomyces cerevisiaeBataille, Alain R. 02 1900 (has links)
La chromatine est plus qu’un système d’empaquetage de l’ADN ; elle est le support de toutes les réactions liées à l’ADN dans le noyau des cellules eucaryotes et participe au contrôle de l’accès de l’ARN polymérase II (ARNPolII) à l’ADN. Responsable de la transcription de tous les ARNm des cellules eucaryotes, l’ARNPolII doit, suivant son recrutement aux promoteurs des gènes, transcrire l’ADN en traversant la matrice chromatinienne. Grâce au domaine C-terminal (CTD) de sa sous-unité Rpb1, elle coordonne la maturation de l’ARNm en cours de synthèse ainsi que les modifications de la chromatine, concomitantes à la transcription. Cette thèse s’intéresse à deux aspects de la transcription : la matrice, avec la localisation de la variante d’histone H2A.Z, et la machinerie de transcription avec le cycle de phosphorylation du CTD de l’ARNPolII.
Suivant l’introduction, le chapitre 2 de cette thèse constitue un protocole détaillé et annoté de la technique de ChIP-chip, chez la levure Saccharomyces cerevisiae. Cette technique phare dans l’étude in vivo des phénomènes liés à l’ADN a grandement facilité l’étude du rôle de la chromatine dans les phénomènes nucléaires, en permettant de localiser sur le génome les marques et les variantes d’histones. Ce chapitre souligne l’importance de contrôles adéquats, spécifiques à l’étude de la chromatine.
Au chapitre 3, grâce à la méthode de ChIP-chip, la variante d’histone H2A.Z est cartographiée au génome de la levure Saccharomyces cerevisiae avec une résolution d’environ 300 paires de bases. Nos résultats montrent que H2A.Z orne un à deux nucléosomes au promoteur de la majorité des gènes. L’enrichissement de H2A.Z est anticorrélé à la transcription et nos résultats suggèrent qu’elle prépare la chromatine pour l’activation des gènes. De plus H2A.Z semble réguler la localisation des nucléosomes.
Le chapitre suivant s’intéresse à la transcription sous l’angle de la machinerie de transcription en se focalisant sur le cycle de phosphorylation de l’ARN polymérase II. Le domaine C-terminal de sa plus large sous-unité est formé de répétitions d’un heptapeptide YSPTSPS dont les résidus peuvent être modifiés au cours de la transcription. Cette étude localise les marques de phosphorylation des trois résidus sérine de manière systématique dans des souches mutantes des kinases et phosphatases. Nos travaux confirment le profil universel des marques de phosphorylations aux gènes transcrits. Appuyés par des essais in vitro, ils révèlent l’interaction complexe des enzymes impliqués dans la phosphorylation, et identifient Ssu72 comme la phosphatase de la sérine 7. Cet article appuie également la notion de « variantes » des marques de phosphorylation bien que leur étude spécifique s’avère encore difficile.
La discussion fait le point sur les travaux qui ont suivi ces articles, et sur les expériences excitantes en cours dans notre laboratoire. / Chromatin is more than just the eucaryotic DNA packaging system; it is the substrate of all reactions involving DNA in eukaryotic cells and actively regulates RNA Polymerase II (RNAPolII) access to DNA. Responsible for all mRNA transcription in eucaryotes, the RNAPolII must, following its recruitment to the pre-initiation complex, overcome the chromatin barrier in order to transcribe genes. The RNAPolII CTD allows for the co-transcriptional coordination of mRNA maturation and chromatin modifications. The work covered in this thesis addresses two aspects of transcription: the chromatin substrate, with the localization of H2A variant, H2A.Z, and the transcription complex with the phosphorylation cycle of the RNAPolII CTD.
Following the introduction, chapter 2 constitutes a detailed and annotated Saccharomyces cerevisiae ChIP-chip protocol, from the culture to the hybridization of the array, with an emphasis on the proper controls required for chromatin study. This technique, extremely powerful for the in vivo study of all DNA transactions, leads to a better understanding of chromatin function in nuclear phenomena, thanks to the localization of histone variants and modifications.
The third chapter maps the H2A.Z variant across the yeast genome at ~300 base pairs resolution using ChIP-chip. Our data shows that H2A.Z is incorporated into one or two promoter-bound nucleosomes at the majority of genes. H2A.Z enrichment is anticorrelated with transcription, and the results suggest that it configures chromatin structure to poise genes for transcriptional activation. Furthermore, we have shown that H2A.Z can regulate nucleosome positioning.
The next chapter focuses on the transcription machinery and, more precisely, on the phosphorylation cycle of RNAPolII. The CTD contains repetitions of a heptapeptide (YSPTSPS) on which all serines are differentially phosphorylated along genes in a prescribed pattern during the transcription cycle. Here, we systematically profiled the location of the RNAPII phospho-isoforms in wild-type cells and mutants for most CTD modifying enzymes. The results provide evidence for a uniform CTD cycle across genes. Together with results from in vitro assays, these data reveal a complex interplay between the modifying enzymes, identify Ssu72 as the Ser7 phosphatase and show that proline isomerization is a key regulator of CTD dephosphorylation at the end of genes. Moreover, it reinforces the notion of variants of the phosphorylation marks, even though the exact nature of the variant is still difficult to identify.
The discussion introduces the studies that followed this work, including new projects conceived in our lab.
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Étude de la variante d’histone H2A.Z et du cycle de phosphorylation de l’ARN polymérase II chez Saccharomyces cerevisiaeBataille, Alain R. 02 1900 (has links)
La chromatine est plus qu’un système d’empaquetage de l’ADN ; elle est le support de toutes les réactions liées à l’ADN dans le noyau des cellules eucaryotes et participe au contrôle de l’accès de l’ARN polymérase II (ARNPolII) à l’ADN. Responsable de la transcription de tous les ARNm des cellules eucaryotes, l’ARNPolII doit, suivant son recrutement aux promoteurs des gènes, transcrire l’ADN en traversant la matrice chromatinienne. Grâce au domaine C-terminal (CTD) de sa sous-unité Rpb1, elle coordonne la maturation de l’ARNm en cours de synthèse ainsi que les modifications de la chromatine, concomitantes à la transcription. Cette thèse s’intéresse à deux aspects de la transcription : la matrice, avec la localisation de la variante d’histone H2A.Z, et la machinerie de transcription avec le cycle de phosphorylation du CTD de l’ARNPolII.
Suivant l’introduction, le chapitre 2 de cette thèse constitue un protocole détaillé et annoté de la technique de ChIP-chip, chez la levure Saccharomyces cerevisiae. Cette technique phare dans l’étude in vivo des phénomènes liés à l’ADN a grandement facilité l’étude du rôle de la chromatine dans les phénomènes nucléaires, en permettant de localiser sur le génome les marques et les variantes d’histones. Ce chapitre souligne l’importance de contrôles adéquats, spécifiques à l’étude de la chromatine.
Au chapitre 3, grâce à la méthode de ChIP-chip, la variante d’histone H2A.Z est cartographiée au génome de la levure Saccharomyces cerevisiae avec une résolution d’environ 300 paires de bases. Nos résultats montrent que H2A.Z orne un à deux nucléosomes au promoteur de la majorité des gènes. L’enrichissement de H2A.Z est anticorrélé à la transcription et nos résultats suggèrent qu’elle prépare la chromatine pour l’activation des gènes. De plus H2A.Z semble réguler la localisation des nucléosomes.
Le chapitre suivant s’intéresse à la transcription sous l’angle de la machinerie de transcription en se focalisant sur le cycle de phosphorylation de l’ARN polymérase II. Le domaine C-terminal de sa plus large sous-unité est formé de répétitions d’un heptapeptide YSPTSPS dont les résidus peuvent être modifiés au cours de la transcription. Cette étude localise les marques de phosphorylation des trois résidus sérine de manière systématique dans des souches mutantes des kinases et phosphatases. Nos travaux confirment le profil universel des marques de phosphorylations aux gènes transcrits. Appuyés par des essais in vitro, ils révèlent l’interaction complexe des enzymes impliqués dans la phosphorylation, et identifient Ssu72 comme la phosphatase de la sérine 7. Cet article appuie également la notion de « variantes » des marques de phosphorylation bien que leur étude spécifique s’avère encore difficile.
La discussion fait le point sur les travaux qui ont suivi ces articles, et sur les expériences excitantes en cours dans notre laboratoire. / Chromatin is more than just the eucaryotic DNA packaging system; it is the substrate of all reactions involving DNA in eukaryotic cells and actively regulates RNA Polymerase II (RNAPolII) access to DNA. Responsible for all mRNA transcription in eucaryotes, the RNAPolII must, following its recruitment to the pre-initiation complex, overcome the chromatin barrier in order to transcribe genes. The RNAPolII CTD allows for the co-transcriptional coordination of mRNA maturation and chromatin modifications. The work covered in this thesis addresses two aspects of transcription: the chromatin substrate, with the localization of H2A variant, H2A.Z, and the transcription complex with the phosphorylation cycle of the RNAPolII CTD.
Following the introduction, chapter 2 constitutes a detailed and annotated Saccharomyces cerevisiae ChIP-chip protocol, from the culture to the hybridization of the array, with an emphasis on the proper controls required for chromatin study. This technique, extremely powerful for the in vivo study of all DNA transactions, leads to a better understanding of chromatin function in nuclear phenomena, thanks to the localization of histone variants and modifications.
The third chapter maps the H2A.Z variant across the yeast genome at ~300 base pairs resolution using ChIP-chip. Our data shows that H2A.Z is incorporated into one or two promoter-bound nucleosomes at the majority of genes. H2A.Z enrichment is anticorrelated with transcription, and the results suggest that it configures chromatin structure to poise genes for transcriptional activation. Furthermore, we have shown that H2A.Z can regulate nucleosome positioning.
The next chapter focuses on the transcription machinery and, more precisely, on the phosphorylation cycle of RNAPolII. The CTD contains repetitions of a heptapeptide (YSPTSPS) on which all serines are differentially phosphorylated along genes in a prescribed pattern during the transcription cycle. Here, we systematically profiled the location of the RNAPII phospho-isoforms in wild-type cells and mutants for most CTD modifying enzymes. The results provide evidence for a uniform CTD cycle across genes. Together with results from in vitro assays, these data reveal a complex interplay between the modifying enzymes, identify Ssu72 as the Ser7 phosphatase and show that proline isomerization is a key regulator of CTD dephosphorylation at the end of genes. Moreover, it reinforces the notion of variants of the phosphorylation marks, even though the exact nature of the variant is still difficult to identify.
The discussion introduces the studies that followed this work, including new projects conceived in our lab.
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RNA Exosome & Chromatin: The Yin & Yang of Transcription: A DissertationRege, Mayuri 12 November 2015 (has links)
Eukaryotic genomes can produce two types of transcripts: protein-coding and non-coding RNAs (ncRNAs). Cryptic ncRNA transcripts are bona fide RNA Pol II products that originate from bidirectional promoters, yet they are degraded by the RNA exosome. Such pervasive transcription is prevalent across eukaryotes, yet its regulation and function is poorly understood.
We hypothesized that chromatin architecture at cryptic promoters may regulate ncRNA transcription. Nucleosomes that flank promoters are highly enriched in two histone marks: H3-K56Ac and the variant H2A.Z, which make nucleosomes highly dynamic. These histone modifications are present at a majority of promoters and their stereotypic pattern is conserved from yeast to mammals, suggesting their evolutionary importance. Although required for inducing a handful of genes, their contribution to steady-state transcription has remained elusive. In this work, we set out to understand if dynamic nucleosomes regulate cryptic transcription and how this is coordinated with the RNA exosome.
Remarkably, we find that H3-K56Ac promotes RNA polymerase II occupancy at a large number of protein coding and noncoding loci, yet neither histone mark has a significant impact on steady state mRNA levels in budding yeast. Instead, broad effects of H3-K56Ac or H2A.Z on levels of both coding and ncRNAs are only revealed in the absence of the nuclear RNA exosome. We show that H2A.Z functions with H3-K56Ac in chromosome folding, facilitating formation of Chromosomal Interaction Domains (CIDs). Our study suggests that H2A.Z and H3-K56Ac work in concert with the RNA exosome to control mRNA and ncRNA levels, perhaps in part by regulating higher order chromatin structures. Together, these chromatin factors achieve a balance of RNA exosome activity (yin; negative) and Pol II (yang; positive) to maintain transcriptional homeostasis.
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Characterization of the contribution of the CHD chromatin remodeler PKL to chromatin modification and gene expression in <i>Arabidopsis thaliana</i>Jiaxin Long (16021247) 12 October 2023 (has links)
<p dir="ltr">H3K27me3 is a transcriptional repressive epigenetic mark that plays vital roles in many biological processes in <i>Arabidopsis thaliana</i>. A number of biochemical and functional characterizations of PKL, an ATP-dependent CHD chromatin remodeler, suggest that PKL contributes to maintain the homeostasis of H3K27me3. To identify other factors that act with PKL together to contribute to the homeostasis of H3K27me3, we undertook an EMS-mutagenesis screen for <i>pkl</i>-associated phenotypes. This genetic screen suggests that PKL may contribute to maintaining the homeostasis of H3K27me3 in an H2A.Z associated or a Mediator associated pathway.</p><p dir="ltr">Here, we took advantage of a combined genetic and bioinformatic method to characterize the contribution of PKL in these two pathways as described above. Our analysis revealed a robust genetic interaction between <i>HTA9</i>, <i>HTA11</i>, and <i>PKL</i> in maintaining proper H2A.Z distribution and enrichment of H3K27me3. In addition, the characterization also sheds light on unexpected roles of PKL in promoting the homeostasis of H3K4me3 and acting with histone demethylases to promote removal of H3K27me3 in an H2A.Z dependent manner. Furthermore, our result also raised the possibility that the tail module of the Mediator complex also plays a critical role in the homeostasis of H3K27me3. While we were examining <i>PKL</i>-dependent chromatin features, we largely optimized the protocol for preparation ChIP-seq samples and libraries and implemented a gene-centric ChIP-seq bioinformatics pipeline for providing robust analysis.</p><p dir="ltr">Ultimately, the work presented in this thesis highlights several divergent pathways that PKL contributes to maintain chromatin homeostasis. By and large, the combined observation from this thesis advances our knowledge of how PKL interacts with other chromatin-associated machineries together to maintain proper epigenetic states and promote other more emergent DNA-templated processes, including replication and transcription.</p>
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