Your search keyword '"Hiratani I"' showing total 36 results

1. Chromosome Engineering Allows the Efficient Isolation of Vertebrate Neocentromeres

Author

Shang, W. H., Hori, T., Martins, N. M., Toyoda, A., Misu, S., Monma, N., Hiratani, I., Maeshima, K., Ikeo, K., Fujiyama, A., Kimura, Hiroshi, Earnshaw, W. C., and Fukagawa, T.

Subjects

DNA Replication, Chromosome engineering, Chromatin Immunoprecipitation, Neocentromere, Transcription, Genetic, Chromosomal Proteins, Non-Histone, Centromere, Autoantigens/genetics, Autoantigens, General Biochemistry, Genetics and Molecular Biology, Article, Chromosomes, Cell Line, Epigenesis, Genetic, Chromosomal Proteins, Non-Histone/genetics, Chromosomes/*genetics, 03 medical and health sciences, Histone H3, 0302 clinical medicine, Animals, Molecular Biology, 030304 developmental biology, Genetics, 0303 health sciences, Replication timing, biology, Base Sequence, DNA replication, Cell Biology, Sequence Analysis, DNA, DNA Methylation, Cell biology, Chickens/*genetics, Histone, Centromere/*genetics/metabolism, biology.protein, Genetic Engineering, Chromatin immunoprecipitation, Chickens, 030217 neurology & neurosurgery, Centromere Protein A, Developmental Biology

Abstract

Summary Centromeres are specified by sequence-independent epigenetic mechanisms in most organisms. Rarely, centromere repositioning results in neocentromere formation at ectopic sites. However, the mechanisms governing how and where neocentromeres form are unknown. Here, we established a chromosome-engineering system in chicken DT40 cells that allowed us to efficiently isolate neocentromere-containing chromosomes. Neocentromeres appear to be structurally and functionally equivalent to native centromeres. Chromatin immunoprecipitation sequencing (ChIP-seq) analysis with 18 neocentromeres revealed that the centromere-specific histone H3 variant CENP-A occupies an ∼40 kb region at each neocentromere, which has no preference for specific DNA sequence motifs. Furthermore, we found that neocentromeres were not associated with histone modifications H3K9me3, H3K4me2, and H3K36me3 or with early replication timing. Importantly, low but significant levels of CENP-A are detected around endogenous centromeres, which are capable of seeding neocentromere assembly if the centromere core is removed. In summary, our experimental system provides valuable insights for understanding how neocentromeres form., Graphical Abstract Highlights ► Chromosome engineering efficiently generates neocentromeres in chicken DT40 cells ► CENP-A reproducibly occupies an ∼40 kb genomic region at each neocentromere ► Nonkinetochore CENP-A appears to function as a seed for neocentromere assembly, Centromeres are specified by sequence-independent epigenetic mechanisms. Shang et al. generated a collection of chicken neocentromeres in DT40 cells. Their analysis indicates that neocentromere formation does not correlate with the expected histone modifications or with replication timing, but rather depends on the histone H3 variant CENP-A to seed assembly.

Published

2013

2. Space and Time in the Nucleus: Developmental Control of Replication Timing and Chromosome Architecture

Author

Gilbert, D. M., primary, Takebayashi, S.- I., additional, Ryba, T., additional, Lu, J., additional, Pope, B. D., additional, Wilson, K. A., additional, and Hiratani, I., additional

Published

2010

3. Requirements of Lim1, a Drosophila LIM-homeobox gene, for normal leg and antennal development

Author

Tsuji, T., primary, Sato, A., additional, Hiratani, I., additional, Taira, M., additional, Saigo, K., additional, and Kojima, T., additional

Published

2000

4. ReplicationDomain: a visualization tool and comparative database for genome-wide replication timing data

Author

Yokochi Tomoki, Ryba Tyrone, Hiratani Ichiro, Stuy Alexander, Weddington Nodin, and Gilbert David M

Subjects

Computer applications to medicine. Medical informatics, R858-859.7, Biology (General), QH301-705.5

Abstract

Abstract Background Eukaryotic DNA replication is regulated at the level of large chromosomal domains (0.5–5 megabases in mammals) within which replicons are activated relatively synchronously. These domains replicate in a specific temporal order during S-phase and our genome-wide analyses of replication timing have demonstrated that this temporal order of domain replication is a stable property of specific cell types. Results We have developed ReplicationDomain http://www.replicationdomain.org as a web-based database for analysis of genome-wide replication timing maps (replication profiles) from various cell lines and species. This database also provides comparative information of transcriptional expression and is configured to display any genome-wide property (for instance, ChIP-Chip or ChIP-Seq data) via an interactive web interface. Our published microarray data sets are publicly available. Users may graphically display these data sets for a selected genomic region and download the data displayed as text files, or alternatively, download complete genome-wide data sets. Furthermore, we have implemented a user registration system that allows registered users to upload their own data sets. Upon uploading, registered users may choose to: (1) view their data sets privately without sharing; (2) share with other registered users; or (3) make their published or "in press" data sets publicly available, which can fulfill journal and funding agencies' requirements for data sharing. Conclusion ReplicationDomain is a novel and powerful tool to facilitate the comparative visualization of replication timing in various cell types as well as other genome-wide chromatin features and is considerably faster and more convenient than existing browsers when viewing multi-megabase segments of chromosomes. Furthermore, the data upload function with the option of private viewing or sharing of data sets between registered users should be a valuable resource for the scientific community.

Published

2008

5. Embryonic genome instability upon DNA replication timing program emergence.

Author

Takahashi S, Kyogoku H, Hayakawa T, Miura H, Oji A, Kondo Y, Takebayashi SI, Kitajima TS, and Hiratani I

Subjects

Animals, Female, Male, Mice, Blastocyst cytology, Blastocyst metabolism, Chromosome Aberrations drug effects, Chromosome Segregation, DNA Damage drug effects, DNA Repair, S Phase drug effects, S Phase genetics, Single-Cell Analysis, Chromosome Breakpoints, Cell Division, Nucleosides metabolism, Nucleosides pharmacology, DNA-Directed DNA Polymerase metabolism, Multienzyme Complexes metabolism, DNA Replication Timing drug effects, Embryo, Mammalian cytology, Embryo, Mammalian metabolism, Embryo, Mammalian embryology, Embryonic Development genetics, Genomic Instability drug effects, Genomic Instability genetics

Abstract

Faithful DNA replication is essential for genome integrity 1-4 . Under-replicated DNA leads to defects in chromosome segregation, which are common during embryogenesis 5-8 . However, the regulation of DNA replication remains poorly understood in early mammalian embryos. Here we constructed a single-cell genome-wide DNA replication atlas of pre-implantation mouse embryos and identified an abrupt replication program switch accompanied by a transient period of genomic instability. In 1- and 2-cell embryos, we observed the complete absence of a replication timing program, and the entire genome replicated gradually and uniformly using extremely slow-moving replication forks. In 4-cell embryos, a somatic-cell-like replication timing program commenced abruptly. However, the fork speed was still slow, S phase was extended, and markers of replication stress, DNA damage and repair increased. This was followed by an increase in break-type chromosome segregation errors specifically during the 4-to-8-cell division with breakpoints enriched in late-replicating regions. These errors were rescued by nucleoside supplementation, which accelerated fork speed and reduced the replication stress. By the 8-cell stage, forks gained speed, S phase was no longer extended and chromosome aberrations decreased. Thus, a transient period of genomic instability exists during normal mouse development, preceded by an S phase lacking coordination between replisome-level regulation and megabase-scale replication timing regulation, implicating a link between their coordination and genome stability., (© 2024. The Author(s).)

Published

2024

6. A feedback loop that drives cell death and proliferation and its defect in intestinal stem cells.

Author

Sulekh S, Ikegawa Y, Naito S, Oji A, Hiratani I, and Yoo SK

Subjects

Animals, Feedback, Inhibitor of Apoptosis Proteins metabolism, Cell Death, Drosophila metabolism, Caspases metabolism, Cell Proliferation genetics, Stem Cells metabolism, Drosophila Proteins genetics, Drosophila Proteins metabolism

Abstract

Cell death and proliferation are at a glance dichotomic events, but occasionally coupled. Caspases, traditionally known to execute apoptosis, play non-apoptotic roles, but their exact mechanism remains elusive. Here, using Drosophila intestinal stem cells (ISCs), we discovered that activation of caspases induces massive cell proliferation rather than cell death. We elucidate that a positive feedback circuit exists between caspases and JNK, which can simultaneously drive cell proliferation and cell death. In ISCs, signalling from JNK to caspases is defective, which skews the balance towards proliferation. Mechanistically, two-tiered regulation of the DIAP1 inhibitor rpr , through its transcription and its protein localization, exists. This work provides a conceptual framework that explains how caspases perform apoptotic and non-apoptotic functions in vivo and how ISCs accomplish their resistance to cell death., (© 2024 Sulekh et al.)

Published

2024

7. Replication dynamics identifies the folding principles of the inactive X chromosome.

Author

Poonperm R, Ichihara S, Miura H, Tanigawa A, Nagao K, Obuse C, Sado T, and Hiratani I

Subjects

X Chromosome Inactivation, DNA Replication, Heterochromatin genetics, X Chromosome genetics

Abstract

Chromosome-wide late replication is an enigmatic hallmark of the inactive X chromosome (Xi). How it is established and what it represents remains obscure. By single-cell DNA replication sequencing, here we show that the entire Xi is reorganized to replicate rapidly and uniformly in late S-phase during X-chromosome inactivation (XCI), reflecting its relatively uniform structure revealed by 4C-seq. Despite this uniformity, only a subset of the Xi became earlier replicating in SmcHD1-mutant cells. In the mutant, these domains protruded out of the Xi core, contacted each other and became transcriptionally reactivated. 4C-seq suggested that they constituted the outermost layer of the Xi even before XCI and were rich in escape genes. We propose that this default positioning forms the basis for their inherent heterochromatin instability in cells lacking the Xi-binding protein SmcHD1 or exhibiting XCI escape. These observations underscore the importance of 3D genome organization for heterochromatin stability and gene regulation., (© 2023. The Author(s).)

Published

2023

8. Epigenetic plasticity safeguards heterochromatin configuration in mammals.

Author

Fukuda K, Shimi T, Shimura C, Ono T, Suzuki T, Onoue K, Okayama S, Miura H, Hiratani I, Ikeda K, Okada Y, Dohmae N, Yonemura S, Inoue A, Kimura H, and Shinkai Y

Subjects

Animals, Histones metabolism, Lysine metabolism, Mammals genetics, Methylation, Histone Methyltransferases metabolism, Epigenesis, Genetic, Heterochromatin genetics

Abstract

Heterochromatin is a key architectural feature of eukaryotic chromosomes critical for cell type-specific gene expression and genome stability. In the mammalian nucleus, heterochromatin segregates from transcriptionally active genomic regions and exists in large, condensed, and inactive nuclear compartments. However, the mechanisms underlying the spatial organization of heterochromatin need to be better understood. Histone H3 lysine 9 trimethylation (H3K9me3) and lysine 27 trimethylation (H3K27me3) are two major epigenetic modifications that enrich constitutive and facultative heterochromatin, respectively. Mammals have at least five H3K9 methyltransferases (SUV39H1, SUV39H2, SETDB1, G9a and GLP) and two H3K27 methyltransferases (EZH1 and EZH2). In this study, we addressed the role of H3K9 and H3K27 methylation in heterochromatin organization using a combination of mutant cells for five H3K9 methyltransferases and an EZH1/2 dual inhibitor, DS3201. We showed that H3K27me3, which is normally segregated from H3K9me3, was redistributed to regions targeted by H3K9me3 after the loss of H3K9 methylation and that the loss of both H3K9 and H3K27 methylation resulted in impaired condensation and spatial organization of heterochromatin. Our data demonstrate that the H3K27me3 pathway safeguards heterochromatin organization after the loss of H3K9 methylation in mammalian cells., (© The Author(s) 2023. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2023

9. Large-Scale Chromatin Rearrangements in Cancer.

Author

Yamaguchi K, Chen X, Oji A, Hiratani I, and Defossez PA

Abstract

Epigenetic abnormalities are extremely widespread in cancer. Some of them are mere consequences of transformation, but some actively contribute to cancer initiation and progression; they provide powerful new biological markers, as well as new targets for therapies. In this review, we examine the recent literature and focus on one particular aspect of epigenome deregulation: large-scale chromatin changes, causing global changes of DNA methylation or histone modifications. After a brief overview of the one-dimension (1D) and three-dimension (3D) epigenome in healthy cells and of its homeostasis mechanisms, we use selected examples to describe how many different events (mutations, changes in metabolism, and infections) can cause profound changes to the epigenome and fuel cancer. We then present the consequences for therapies and briefly discuss the role of single-cell approaches for the future progress of the field.

Published

2022

10. Cell cycle dynamics and developmental dynamics of the 3D genome: toward linking the two timescales.

Author

Miura H and Hiratani I

Subjects

Animals, Cell Cycle genetics, Cell Nucleus genetics, Chromatin genetics, Interphase genetics, Mammals genetics, Chromosomes genetics, Genome genetics

Abstract

In the mammalian cell nucleus, chromosomes are folded differently in interphase and mitosis. Interphase chromosomes are relatively decondensed and display at least two unique layers of higher-order organization: topologically associating domains (TADs) and cell-type-specific A/B compartments, which correlate well with early/late DNA replication timing (RT). In mitosis, these structures rapidly disappear but are gradually reconstructed during G1 phase, coincident with the establishment of the RT program. However, these structures also change dynamically during cell differentiation and reprogramming, and yet we are surprisingly ignorant about the relationship between their cell cycle dynamics and developmental dynamics. In this review, we summarize the recent findings on this topic, discuss how these two processes might be coordinated with each other and its potential significance., (Copyright © 2022 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published

2022

11. SAF-A promotes origin licensing and replication fork progression to ensure robust DNA replication.

Author

Connolly C, Takahashi S, Miura H, Hiratani I, Gilbert N, Donaldson AD, and Hiraga SI

Subjects

Chromatin genetics, G1 Phase, Replication Origin genetics, S Phase genetics, Chromosomes, DNA Replication

Abstract

The organisation of chromatin is closely intertwined with biological activities of chromosome domains, including transcription and DNA replication status. Scaffold-attachment factor A (SAF-A), also known as heterogeneous nuclear ribonucleoprotein U (HNRNPU), contributes to the formation of open chromatin structure. Here, we demonstrate that SAF-A promotes the normal progression of DNA replication and enables resumption of replication after inhibition. We report that cells depleted of SAF-A show reduced origin licensing in G1 phase and, consequently, reduced origin activation frequency in S phase. Replication forks also progress less consistently in cells depleted of SAF-A, contributing to reduced DNA synthesis rate. Single-cell replication timing analysis revealed two distinct effects of SAF-A depletion: first, the boundaries between early- and late-replicating domains become more blurred; and second, SAF-A depletion causes replication timing changes that tend to bring regions of discordant domain compartmentalisation and replication timing into concordance. Associated with these defects, SAF-A-depleted cells show elevated formation of phosphorylated histone H2AX (γ-H2AX) and tend to enter quiescence. Overall, we find that SAF-A protein promotes robust DNA replication to ensure continuing cell proliferation., Competing Interests: Competing interests The authors declare no competing or financial interests., (© 2022. Published by The Company of Biologists Ltd.)

Published

2022

12. Highly rigid H3.1/H3.2-H3K9me3 domains set a barrier for cell fate reprogramming in trophoblast stem cells.

Author

Hada M, Miura H, Tanigawa A, Matoba S, Inoue K, Ogonuki N, Hirose M, Watanabe N, Nakato R, Fujiki K, Hasegawa A, Sakashita A, Okae H, Miura K, Shikata D, Arima T, Shirahige K, Hiratani I, and Ogura A

Subjects

Animals, Cell Differentiation genetics, Female, Mammals, Mice, Placenta, Pregnancy, Stem Cells, Histones genetics, Histones metabolism, Trophoblasts metabolism

Abstract

The placenta is a highly evolved, specialized organ in mammals. It differs from other organs in that it functions only for fetal maintenance during gestation. Therefore, there must be intrinsic mechanisms that guarantee its unique functions. To address this question, we comprehensively analyzed epigenomic features of mouse trophoblast stem cells (TSCs). Our genome-wide, high-throughput analyses revealed that the TSC genome contains large-scale (>1-Mb) rigid heterochromatin architectures with a high degree of histone H3.1/3.2-H3K9me3 accumulation, which we termed TSC-defined highly heterochromatinized domains (THDs). Importantly, depletion of THDs by knockdown of CAF1, an H3.1/3.2 chaperone, resulted in down-regulation of TSC markers, such as Cdx2 and Elf5 , and up-regulation of the pluripotent marker Oct3/4 , indicating that THDs maintain the trophoblastic nature of TSCs. Furthermore, our nuclear transfer technique revealed that THDs are highly resistant to genomic reprogramming. However, when H3K9me3 was removed, the TSC genome was fully reprogrammed, giving rise to the first TSC cloned offspring. Interestingly, THD-like domains are also present in mouse and human placental cells in vivo, but not in other cell types. Thus, THDs are genomic architectures uniquely developed in placental lineage cells, which serve to protect them from fate reprogramming to stably maintain placental function., (© 2022 Hada et al.; Published by Cold Spring Harbor Laboratory Press.)

Published

2022

13. Regulation of mammalian 3D genome organization and histone H3K9 dimethylation by H3K9 methyltransferases.

Author

Fukuda K, Shimura C, Miura H, Tanigawa A, Suzuki T, Dohmae N, Hiratani I, and Shinkai Y

Subjects

Animals, Chromatin chemistry, Chromatin genetics, Fibroblasts cytology, Genome, Histone-Lysine N-Methyltransferase genetics, Histones chemistry, Histones genetics, Lysine chemistry, Lysine genetics, Mice, Mouse Embryonic Stem Cells cytology, Chromatin metabolism, DNA Methylation, Fibroblasts metabolism, Histone-Lysine N-Methyltransferase metabolism, Histones metabolism, Lysine metabolism, Mouse Embryonic Stem Cells metabolism

Abstract

Histone H3 lysine 9 dimethylation (H3K9me2) is a highly conserved silencing epigenetic mark. Chromatin marked with H3K9me2 forms large domains in mammalian cells and overlaps well with lamina-associated domains and the B compartment defined by Hi-C. However, the role of H3K9me2 in 3-dimensional (3D) genome organization remains unclear. Here, we investigated genome-wide H3K9me2 distribution, transcriptome, and 3D genome organization in mouse embryonic stem cells following the inhibition or depletion of H3K9 methyltransferases (MTases): G9a, GLP, SETDB1, SUV39H1, and SUV39H2. We show that H3K9me2 is regulated by all five MTases; however, H3K9me2 and transcription in the A and B compartments are regulated by different MTases. H3K9me2 in the A compartments is primarily regulated by G9a/GLP and SETDB1, while H3K9me2 in the B compartments is regulated by all five MTases. Furthermore, decreased H3K9me2 correlates with changes to more active compartmental state that accompanied transcriptional activation. Thus, H3K9me2 contributes to inactive compartment setting.

Published

2021

14. Dynamics of transcription-mediated conversion from euchromatin to facultative heterochromatin at the Xist promoter by Tsix.

Author

Ohhata T, Yamazawa K, Miura-Kamio A, Takahashi S, Sakai S, Tamura Y, Uchida C, Kitagawa K, Niida H, Hiratani I, Kobayashi H, Kimura H, Wutz A, and Kitagawa M

Subjects

Animals, CCCTC-Binding Factor metabolism, DNA Methylation genetics, Epigenesis, Genetic, Fibroblasts cytology, Fibroblasts metabolism, Gene Silencing, Germ Layers cytology, Histones metabolism, Mice, Nucleosomes metabolism, Protein Processing, Post-Translational, RNA, Long Noncoding metabolism, Stem Cells metabolism, YY1 Transcription Factor metabolism, Euchromatin metabolism, Heterochromatin metabolism, Promoter Regions, Genetic, RNA, Long Noncoding genetics, Transcription, Genetic

Abstract

The fine-scale dynamics from euchromatin (EC) to facultative heterochromatin (fHC) has remained largely unclear. Here, we focus on Xist and its silencing initiator Tsix as a paradigm of transcription-mediated conversion from EC to fHC. In mouse epiblast stem cells, induction of Tsix recapitulates the conversion at the Xist promoter. Investigating the dynamics reveals that the conversion proceeds in a stepwise manner. Initially, a transient opened chromatin structure is observed. In the second step, gene silencing is initiated and dependent on Tsix, which is reversible and accompanied by simultaneous changes in multiple histone modifications. At the last step, maintenance of silencing becomes independent of Tsix and irreversible, which correlates with occupation of the -1 position of the transcription start site by a nucleosome and initiation of DNA methylation introduction. This study highlights the hierarchy of multiple chromatin events upon stepwise gene silencing establishment., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2021 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2021

15. The Temporal Order of DNA Replication Shaped by Mammalian DNA Methyltransferases.

Author

Takebayashi SI, Ryba T, Wimbish K, Hayakawa T, Sakaue M, Kuriya K, Takahashi S, Ogata S, Hiratani I, Okumura K, Okano M, and Ogata M

Subjects

Animals, Chromosomes, Mammalian metabolism, DNA Methylation genetics, Genome, Heterochromatin metabolism, Histones metabolism, Lysine metabolism, Methylation, Mice, Mice, Knockout, Mouse Embryonic Stem Cells metabolism, Transcription, Genetic, DNA metabolism, DNA Replication Timing genetics, Mammals metabolism, Methyltransferases metabolism

Abstract

Multiple epigenetic pathways underlie the temporal order of DNA replication (replication timing) in the contexts of development and disease. DNA methylation by DNA methyltransferases (Dnmts) and downstream chromatin reorganization and transcriptional changes are thought to impact DNA replication, yet this remains to be comprehensively tested. Using cell-based and genome-wide approaches to measure replication timing, we identified a number of genomic regions undergoing subtle but reproducible replication timing changes in various Dnmt -mutant mouse embryonic stem (ES) cell lines that included a cell line with a drug-inducible Dnmt3a2 expression system. Replication timing within pericentromeric heterochromatin (PH) was shown to be correlated with redistribution of H3K27me3 induced by DNA hypomethylation: Later replicating PH coincided with H3K27me3-enriched regions. In contrast, this relationship with H3K27me3 was not evident within chromosomal arm regions undergoing either early-to-late (EtoL) or late-to-early (LtoE) switching of replication timing upon loss of the Dnmts. Interestingly, Dnmt-sensitive transcriptional up- and downregulation frequently coincided with earlier and later shifts in replication timing of the chromosomal arm regions, respectively. Our study revealed the previously unrecognized complex and diverse effects of the Dnmts loss on the mammalian DNA replication landscape.

Published

2021

16. Microrheology for Hi-C Data Reveals the Spectrum of the Dynamic 3D Genome Organization.

Author

Shinkai S, Sugawara T, Miura H, Hiratani I, and Onami S

Subjects

Animals, Cell Nucleus, DNA, Mice, Mouse Embryonic Stem Cells, Chromatin genetics, Chromosomes genetics

Abstract

The one-dimensional information of genomic DNA is hierarchically packed inside the eukaryotic cell nucleus and organized in a three-dimensional (3D) space. Genome-wide chromosome conformation capture (Hi-C) methods have uncovered the 3D genome organization and revealed multiscale chromatin domains of compartments and topologically associating domains (TADs). Moreover, single-nucleosome live-cell imaging experiments have revealed the dynamic organization of chromatin domains caused by stochastic thermal fluctuations. However, the mechanism underlying the dynamic regulation of such hierarchical and structural chromatin units within the microscale thermal medium remains unclear. Microrheology is a way to measure dynamic viscoelastic properties coupling between thermal microenvironment and mechanical response. Here, we propose a new, to our knowledge, microrheology for Hi-C data to analyze the dynamic compliance property as a measure of rigidness and flexibility of genomic regions along with the time evolution. Our method allows the conversion of an Hi-C matrix into the spectrum of the dynamic rheological property along the genomic coordinate of a single chromosome. To demonstrate the power of the technique, we analyzed Hi-C data during the neural differentiation of mouse embryonic stem cells. We found that TAD boundaries behave as more rigid nodes than the intra-TAD regions. The spectrum clearly shows the dynamic viscoelasticity of chromatin domain formation at different timescales. Furthermore, we characterized the appearance of synchronous and liquid-like intercompartment interactions in differentiated cells. Together, our microrheology data derived from Hi-C data provide physical insights into the dynamics of the 3D genome organization., (Copyright © 2020 Biophysical Society. Published by Elsevier Inc. All rights reserved.)

Published

2020

17. Multifaceted Hi-C benchmarking: what makes a difference in chromosome-scale genome scaffolding?

Author

Kadota M, Nishimura O, Miura H, Tanaka K, Hiratani I, and Kuraku S

Subjects

Animals, Gene Expression Profiling, High-Throughput Nucleotide Sequencing, In Situ Hybridization, Turtles genetics, Chromatin genetics, Chromosome Mapping methods, Chromosomes genetics, Computational Biology methods, Genomics methods, Software

Abstract

Background: Hi-C is derived from chromosome conformation capture (3C) and targets chromatin contacts on a genomic scale. This method has also been used frequently in scaffolding nucleotide sequences obtained by de novo genome sequencing and assembly, in which the number of resultant sequences rarely converges to the chromosome number. Despite its prevalent use, the sample preparation methods for Hi-C have not been intensively discussed, especially from the standpoint of genome scaffolding., Results: To gain insight into the best practice of Hi-C scaffolding, we performed a multifaceted methodological comparison using vertebrate samples and optimized various factors during sample preparation, sequencing, and computation. As a result, we identified several key factors that helped improve Hi-C scaffolding, including the choice and preparation of tissues, library preparation conditions, the choice of restriction enzyme(s), and the choice of scaffolding program and its usage., Conclusions: This study provides the first comparison of multiple sample preparation kits/protocols and computational programs for Hi-C scaffolding by an academic third party. We introduce a customized protocol designated "inexpensive and controllable Hi-C (iconHi-C) protocol," which incorporates the optimal conditions identified in this study, and demonstrate this technique on chromosome-scale genome sequences of the Chinese softshell turtle Pelodiscus sinensis., (© The Author(s) 2020. Published by Oxford University Press.)

Published

2020

18. The Eleanor ncRNAs activate the topological domain of the ESR1 locus to balance against apoptosis.

Author

Abdalla MOA, Yamamoto T, Maehara K, Nogami J, Ohkawa Y, Miura H, Poonperm R, Hiratani I, Nakayama H, Nakao M, and Saitoh N

Subjects

Antineoplastic Agents, Hormonal pharmacology, Antineoplastic Agents, Hormonal therapeutic use, Apoptosis drug effects, Aromatase Inhibitors pharmacology, Aromatase Inhibitors therapeutic use, Binding Sites genetics, Breast Neoplasms drug therapy, Breast Neoplasms pathology, Chromatin genetics, Chromatin metabolism, Drug Resistance, Neoplasm genetics, Epigenesis, Genetic, Estrogen Receptor alpha metabolism, Estrogens metabolism, Female, Forkhead Box Protein O3 genetics, Forkhead Box Protein O3 metabolism, Genetic Loci genetics, High-Throughput Nucleotide Sequencing, Humans, MCF-7 Cells, Promoter Regions, Genetic genetics, Up-Regulation, Apoptosis genetics, Breast Neoplasms genetics, Estrogen Receptor alpha genetics, Gene Expression Regulation, Neoplastic, RNA, Untranslated metabolism

Abstract

MCF7 cells acquire estrogen-independent proliferation after long-term estrogen deprivation (LTED), which recapitulates endocrine therapy resistance. LTED cells can become primed for apoptosis, but the underlying mechanism is largely unknown. We previously reported that Eleanor non-coding RNAs (ncRNAs) upregulate the ESR1 gene in LTED cells. Here, we show that Eleanors delineate the topologically associating domain (TAD) of the ESR1 locus in the active nuclear compartment of LTED cells. The TAD interacts with another transcriptionally active TAD, which is 42.9 Mb away from ESR1 and contains a gene encoding the apoptotic transcription factor FOXO3. Inhibition of a promoter-associated Eleanor suppresses all genes inside the Eleanor TAD and the long-range interaction between the two TADs, but keeps FOXO3 active to facilitate apoptosis in LTED cells. These data indicate a role of ncRNAs in chromatin domain regulation, which may underlie the apoptosis-prone nature of therapy-resistant breast cancer cells and could be good therapeutic targets.

Published

2019

19. DNA Replication Timing Enters the Single-Cell Era.

Author

Hiratani I and Takahashi S

Subjects

Animals, Gene Expression Regulation, Developmental, Humans, Mammals growth & development, Whole Genome Sequencing, DNA Replication Timing, Mammals genetics, Single-Cell Analysis methods

Abstract

In mammalian cells, DNA replication timing is controlled at the level of megabase (Mb)-sized chromosomal domains and correlates well with transcription, chromatin structure, and three-dimensional (3D) genome organization. Because of these properties, DNA replication timing is an excellent entry point to explore genome regulation at various levels and a variety of studies have been carried out over the years. However, DNA replication timing studies traditionally required at least tens of thousands of cells, and it was unclear whether the replication domains detected by cell population analyses were preserved at the single-cell level. Recently, single-cell DNA replication profiling methods became available, which revealed that the Mb-sized replication domains detected by cell population analyses were actually well preserved in individual cells. In this article, we provide a brief overview of our current knowledge on DNA replication timing regulation in mammals based on cell population studies, outline the findings from single-cell DNA replication profiling, and discuss future directions and challenges.

Published

2019

20. Srf destabilizes cellular identity by suppressing cell-type-specific gene expression programs.

Author

Ikeda T, Hikichi T, Miura H, Shibata H, Mitsunaga K, Yamada Y, Woltjen K, Miyamoto K, Hiratani I, Yamada Y, Hotta A, Yamamoto T, Okita K, and Masui S

Subjects

Actins genetics, Actins metabolism, Animals, Cell Differentiation, Cellular Reprogramming genetics, Chromatin metabolism, Colitis, Ulcerative metabolism, Colitis, Ulcerative pathology, Disease Models, Animal, Female, Gene Expression Regulation, Induced Pluripotent Stem Cells cytology, Male, Metaplasia metabolism, Metaplasia pathology, Mice, Mice, Transgenic, Neural Stem Cells cytology, Pancreas pathology, Serum Response Factor metabolism, Signal Transduction, Trans-Activators genetics, Trans-Activators metabolism, Chromatin chemistry, Colitis, Ulcerative genetics, Induced Pluripotent Stem Cells metabolism, Metaplasia genetics, Neural Stem Cells metabolism, Pancreas metabolism, Serum Response Factor genetics

Abstract

Multicellular organisms consist of multiple cell types. The identity of these cells is primarily maintained by cell-type-specific gene expression programs; however, mechanisms that suppress these programs are poorly defined. Here we show that serum response factor (Srf), a transcription factor that is activated by various extracellular stimuli, can repress cell-type-specific genes and promote cellular reprogramming to pluripotency. Manipulations that decrease β-actin monomer quantity result in the nuclear accumulation of Mkl1 and the activation of Srf, which downregulate cell-type-specific genes and alter the epigenetics of regulatory regions and chromatin organization. Mice overexpressing Srf exhibit various pathologies including an ulcerative colitis-like symptom and a metaplasia-like phenotype in the pancreas. Our results demonstrate an unexpected function of Srf via a mechanism by which extracellular stimuli actively destabilize cell identity and suggest Srf involvement in a wide range of diseases.

Published

2018

21. Epigenetic differences between naïve and primed pluripotent stem cells.

Author

Takahashi S, Kobayashi S, and Hiratani I

Subjects

Animals, Cell Differentiation genetics, Humans, Mice, Blastocyst Inner Cell Mass metabolism, Epigenesis, Genetic, Germ Layers metabolism, Mouse Embryonic Stem Cells metabolism, Pluripotent Stem Cells metabolism

Abstract

It has been 8 years since the concept of naïve and primed pluripotent stem cell states was first proposed. Both are states of pluripotency, but exhibit slightly different properties. The naïve state represents the cellular state of the preimplantation mouse blastocyst inner cell mass, while the primed state is representative of the post-implantation epiblast cells. These two cell types exhibit clearly distinct developmental potential, as evidenced by the fact that naïve cells are able to contribute to blastocyst chimeras, while primed cells cannot. However, the epigenetic differences that underlie the distinct developmental potential of these cell types remain unclear, which is rather surprising given the large amount of active investigation over the years. Elucidating such epigenetic differences should lead to a better understanding of the fundamental properties of these states of pluripotency and the means by which the naïve-to-primed transition occurs, which may provide insights into the essence of stem cell commitment.

Published

2018

22. Chromatin folding and DNA replication inhibition mediated by a highly antitumor-active tetrazolato-bridged dinuclear platinum(II) complex.

Author

Imai R, Komeda S, Shimura M, Tamura S, Matsuyama S, Nishimura K, Rogge R, Matsunaga A, Hiratani I, Takata H, Uemura M, Iida Y, Yoshikawa Y, Hansen JC, Yamauchi K, Kanemaki MT, and Maeshima K

Subjects

Cell Cycle Checkpoints drug effects, Cell Cycle Checkpoints genetics, Cell Line, Tumor, Cell Proliferation drug effects, Cisplatin pharmacology, DNA Damage, DNA Repair, Histones metabolism, Humans, Organoplatinum Compounds chemistry, Tetrazoles chemistry, Transcription, Genetic drug effects, Antineoplastic Agents pharmacology, Chromatin Assembly and Disassembly drug effects, DNA Replication drug effects, Organoplatinum Compounds pharmacology, Tetrazoles pharmacology

Abstract

Chromatin DNA must be read out for various cellular functions, and copied for the next cell division. These processes are targets of many anticancer agents. Platinum-based drugs, such as cisplatin, have been used extensively in cancer chemotherapy. The drug-DNA interaction causes DNA crosslinks and subsequent cytotoxicity. Recently, it was reported that an azolato-bridged dinuclear platinum(II) complex, 5-H-Y, exhibits a different anticancer spectrum from cisplatin. Here, using an interdisciplinary approach, we reveal that the cytotoxic mechanism of 5-H-Y is distinct from that of cisplatin. 5-H-Y inhibits DNA replication and also RNA transcription, arresting cells in the S/G2 phase, and are effective against cisplatin-resistant cancer cells. Moreover, it causes much less DNA crosslinking than cisplatin, and induces chromatin folding. 5-H-Y will expand the clinical applications for the treatment of chemotherapy-insensitive cancers.

Published

2016

23. Replication timing: a fingerprint for cell identity and pluripotency.

Author

Ryba T, Hiratani I, Sasaki T, Battaglia D, Kulik M, Zhang J, Dalton S, and Gilbert DM

Subjects

Animals, Cell Line, Chromatin metabolism, DNA Methylation, Endoderm cytology, Epigenomics, Gene Expression Regulation, Developmental, Histones genetics, Histones metabolism, Humans, Mesoderm cytology, Mice, Monte Carlo Method, Muscle, Smooth cytology, DNA Fingerprinting methods, DNA Replication Timing physiology, Embryonic Stem Cells classification, Pluripotent Stem Cells classification

Abstract

Many types of epigenetic profiling have been used to classify stem cells, stages of cellular differentiation, and cancer subtypes. Existing methods focus on local chromatin features such as DNA methylation and histone modifications that require extensive analysis for genome-wide coverage. Replication timing has emerged as a highly stable cell type-specific epigenetic feature that is regulated at the megabase-level and is easily and comprehensively analyzed genome-wide. Here, we describe a cell classification method using 67 individual replication profiles from 34 mouse and human cell lines and stem cell-derived tissues, including new data for mesendoderm, definitive endoderm, mesoderm and smooth muscle. Using a Monte-Carlo approach for selecting features of replication profiles conserved in each cell type, we identify "replication timing fingerprints" unique to each cell type and apply a k nearest neighbor approach to predict known and unknown cell types. Our method correctly classifies 67/67 independent replication-timing profiles, including those derived from closely related intermediate stages. We also apply this method to derive fingerprints for pluripotency in human and mouse cells. Interestingly, the mouse pluripotency fingerprint overlaps almost completely with previously identified genomic segments that switch from early to late replication as pluripotency is lost. Thereafter, replication timing and transcription within these regions become difficult to reprogram back to pluripotency, suggesting these regions highlight an epigenetic barrier to reprogramming. In addition, the major histone cluster Hist1 consistently becomes later replicating in committed cell types, and several histone H1 genes in this cluster are downregulated during differentiation, suggesting a possible instrument for the chromatin compaction observed during differentiation. Finally, we demonstrate that unknown samples can be classified independently using site-specific PCR against fingerprint regions. In sum, replication fingerprints provide a comprehensive means for cell characterization and are a promising tool for identifying regions with cell type-specific organization.

Published

2011

24. DNA replication timing is maintained genome-wide in primary human myoblasts independent of D4Z4 contraction in FSH muscular dystrophy.

Author

Pope BD, Tsumagari K, Battaglia D, Ryba T, Hiratani I, Ehrlich M, and Gilbert DM

Subjects

Adolescent, Adult, Cells, Cultured, DNA Replication Timing genetics, Female, Humans, Male, Middle Aged, Young Adult, DNA Replication Timing physiology, Muscular Dystrophy, Facioscapulohumeral genetics, Muscular Dystrophy, Facioscapulohumeral metabolism, Myoblasts metabolism, Tandem Repeat Sequences genetics

Abstract

Facioscapulohumeral muscular dystrophy (FSHD) is linked to contraction of an array of tandem 3.3-kb repeats (D4Z4) at 4q35.2 from 11-100 copies to 1-10 copies. The extent to which D4Z4 contraction at 4q35.2 affects overall 4q35.2 chromatin organization remains unclear. Because DNA replication timing is highly predictive of long-range chromatin interactions, we generated genome-wide replication-timing profiles for FSHD and control myogenic precursor cells. We compared non-immortalized myoblasts from four FSHD patients and three control individuals to each other and to a variety of other human cell types. This study also represents the first genome-wide comparison of replication timing profiles in non-immortalized human cell cultures. Myoblasts from both control and FSHD individuals all shared a myoblast-specific replication profile. In contrast, male and female individuals were readily distinguished by monoallelic differences in replication timing at DXZ4 and other regions across the X chromosome affected by X inactivation. We conclude that replication timing is a robust cell-type specific feature that is unaffected by FSHD-related D4Z4 contraction.

Published

2011

25. Evolutionarily conserved replication timing profiles predict long-range chromatin interactions and distinguish closely related cell types.

Author

Ryba T, Hiratani I, Lu J, Itoh M, Kulik M, Zhang J, Schulz TC, Robins AJ, Dalton S, and Gilbert DM

Subjects

Animals, Cell Line, Embryonic Stem Cells metabolism, Humans, Mice, Biological Evolution, Chromatin genetics, DNA Replication

Abstract

To identify evolutionarily conserved features of replication timing and their relationship to epigenetic properties, we profiled replication timing genome-wide in four human embryonic stem cell (hESC) lines, hESC-derived neural precursor cells (NPCs), lymphoblastoid cells, and two human induced pluripotent stem cell lines (hiPSCs), and compared them with related mouse cell types. Results confirm the conservation of coordinately replicated megabase-sized "replication domains" punctuated by origin-suppressed regions. Differentiation-induced replication timing changes in both species occur in 400- to 800-kb units and are similarly coordinated with transcription changes. A surprising degree of cell-type-specific conservation in replication timing was observed across regions of conserved synteny, despite considerable species variation in the alignment of replication timing to isochore GC/LINE-1 content. Notably, hESC replication timing profiles were significantly more aligned to mouse epiblast-derived stem cells (mEpiSCs) than to mouse ESCs. Comparison with epigenetic marks revealed a signature of chromatin modifications at the boundaries of early replicating domains and a remarkably strong link between replication timing and spatial proximity of chromatin as measured by Hi-C analysis. Thus, early and late initiation of replication occurs in spatially separate nuclear compartments, but rarely within the intervening chromatin. Moreover, cell-type-specific conservation of the replication program implies conserved developmental changes in spatial organization of chromatin. Together, our results reveal evolutionarily conserved aspects of developmentally regulated replication programs in mammals, demonstrate the power of replication profiling to distinguish closely related cell types, and strongly support the hypothesis that replication timing domains are spatially compartmentalized structural and functional units of three-dimensional chromosomal architecture.

Published

2010

26. Genome-wide dynamics of replication timing revealed by in vitro models of mouse embryogenesis.

Author

Hiratani I, Ryba T, Itoh M, Rathjen J, Kulik M, Papp B, Fussner E, Bazett-Jones DP, Plath K, Dalton S, Rathjen PD, and Gilbert DM

Subjects

Animals, Cell Differentiation genetics, Cell Line, Chromatin genetics, CpG Islands genetics, Down-Regulation genetics, Embryonic Stem Cells cytology, Epigenesis, Genetic genetics, Female, Gene Expression Regulation, Developmental, Germ Layers growth & development, Homeodomain Proteins genetics, Mice, Nanog Homeobox Protein, Octamer Transcription Factor-3 genetics, Pluripotent Stem Cells cytology, Promoter Regions, Genetic genetics, SOXB1 Transcription Factors genetics, Transcription, Genetic genetics, DNA Replication Timing genetics, Embryonic Development genetics, Genome-Wide Association Study

Abstract

Differentiation of mouse embryonic stem cells (mESCs) is accompanied by changes in replication timing. To explore the relationship between replication timing and cell fate transitions, we constructed genome-wide replication-timing profiles of 22 independent mouse cell lines representing 10 stages of early mouse development, and transcription profiles for seven of these stages. Replication profiles were cell-type specific, with 45% of the genome exhibiting significant changes at some point during development that were generally coordinated with changes in transcription. Comparison of early and late epiblast cell culture models revealed a set of early-to-late replication switches completed at a stage equivalent to the post-implantation epiblast, prior to germ layer specification and down-regulation of key pluripotency transcription factors [POU5F1 (also known as OCT4)/NANOG/SOX2] and coinciding with the emergence of compact chromatin near the nuclear periphery. These changes were maintained in all subsequent lineages (lineage-independent) and involved a group of irreversibly down-regulated genes, at least some of which were repositioned closer to the nuclear periphery. Importantly, many genomic regions of partially reprogrammed induced pluripotent stem cells (piPSCs) failed to re-establish ESC-specific replication-timing and transcription programs. These regions were enriched for lineage-independent early-to-late changes, which in female cells included the inactive X chromosome. Together, these results constitute a comprehensive "fate map" of replication-timing changes during early mouse development. Moreover, they support a model in which a distinct set of replication domains undergoes a form of "autosomal Lyonization" in the epiblast that is difficult to reprogram and coincides with an epigenetic commitment to differentiation prior to germ layer specification.

Published

2010

27. Domain-wide regulation of DNA replication timing during mammalian development.

Author

Pope BD, Hiratani I, and Gilbert DM

Subjects

Animals, Gene Expression Regulation, Developmental, Genome, Humans, Mice, X Chromosome Inactivation, DNA Replication, Mammals genetics

Abstract

Studies of replication timing provide a handle into previously impenetrable higher-order levels of chromosome organization and their plasticity during development. Although mechanisms regulating replication timing are not clear, novel genome-wide studies provide a thorough survey of the extent to which replication timing is regulated during most of the early cell fate transitions in mammals, revealing coordinated changes of a defined set of 400-800 kb chromosomal segments that involve at least half the genome. Furthermore, changes in replication time are linked to changes in sub-nuclear organization and domain-wide transcriptional potential, and tissue-specific replication timing profiles are conserved from mouse to human, suggesting that the program has developmental significance. Hence, these studies have provided a solid foundation for linking megabase level chromosome structure to function, and suggest a central role for replication in domain-level genome organization.

Published

2010

28. G9a selectively represses a class of late-replicating genes at the nuclear periphery.

Author

Yokochi T, Poduch K, Ryba T, Lu J, Hiratani I, Tachibana M, Shinkai Y, and Gilbert DM

Subjects

Animals, Cell Line, Cell Nucleus enzymology, Chromatin metabolism, DNA Methylation, Gene Knockout Techniques, Histone-Lysine N-Methyltransferase genetics, Mice, Promoter Regions, Genetic, Repressor Proteins genetics, Cell Nucleus genetics, DNA Replication, Gene Expression Regulation, Histone-Lysine N-Methyltransferase metabolism, Repressor Proteins metabolism

Abstract

We have investigated the role of the histone methyltransferase G9a in the establishment of silent nuclear compartments. Following conditional knockout of the G9a methyltransferase in mouse ESCs, 167 genes were significantly up-regulated, and no genes were strongly down-regulated. A partially overlapping set of 119 genes were up-regulated after differentiation of G9a-depleted cells to neural precursors. Promoters of these G9a-repressed genes were AT rich and H3K9me2 enriched but H3K4me3 depleted and were not highly DNA methylated. Representative genes were found to be close to the nuclear periphery, which was significantly enriched for G9a-dependent H3K9me2. Strikingly, although 73% of total genes were early replicating, more than 71% of G9a-repressed genes were late replicating, and a strong correlation was found between H3K9me2 and late replication. However, G9a loss did not significantly affect subnuclear position or replication timing of any non-pericentric regions of the genome, nor did it affect programmed changes in replication timing that accompany differentiation. We conclude that G9a is a gatekeeper for a specific set of genes localized within the late replicating nuclear periphery.

Published

2009

29. Replication timing and transcriptional control: beyond cause and effect--part II.

Author

Hiratani I, Takebayashi S, Lu J, and Gilbert DM

Subjects

Animals, Cell Differentiation genetics, Gene Expression Regulation, Humans, Isochores genetics, S Phase genetics, DNA Replication genetics, DNA Replication Timing, Transcription, Genetic genetics

Abstract

Replication timing is frequently discussed superficially in terms of its relationship to transcriptional activity via chromatin structure. However, so little is known about what regulates where and when replication initiates that it has been impossible to identify mechanistic and causal relationships. Moreover, much of our knowledge base has been anecdotal, derived from analyses of a few genes in unrelated cell lines. Recent studies have revisited long-standing hypotheses using genome-wide approaches. In particular, the foundation of this field was recently shored up with incontrovertible evidence that cellular differentiation is accompanied by coordinated changes in replication timing and transcription. These changes accompany subnuclear repositioning, and take place at the level of megabase-sized domains that transcend localized changes in chromatin structure or transcription. Inferring from these results, we propose that there exists a key transition during the middle of S-phase and that changes in replication timing traversing this period are associated with subnuclear repositioning and changes in the activity of certain classes of promoters.

Published

2009

30. Replication timing as an epigenetic mark.

Author

Hiratani I and Gilbert DM

Subjects

Cell Cycle, Cell Differentiation genetics, Time Factors, Transcription, Genetic, DNA Replication genetics, Epigenesis, Genetic

Abstract

Although early replication has long been associated with accessible chromatin, replication timing is not included in most discussions of epigenetic marks. This is partly due to a lack of understanding of the mechanisms behind this association but the issue has also been confounded by studies concluding that there are very few changes in replication timing during development. Recently, the first genome-wide study of replication timing during the course of differentiation revealed extensive changes that were strongly associated with changes in transcriptional activity and subnuclear organization. Domains of temporally coordinate replication delineate discrete units of chromosome structure and function that are characteristic of particular differentiation states. Hence, although we are still a long way from understanding the functional significance of replication timing, it is clear that replication timing is a distinct epigenetic signature of cell differentiation state.

Published

2009

31. ReplicationDomain: a visualization tool and comparative database for genome-wide replication timing data.

Author

Weddington N, Stuy A, Hiratani I, Ryba T, Yokochi T, and Gilbert DM

Subjects

Database Management Systems, Information Storage and Retrieval, User-Computer Interface, Computer Graphics, DNA Replication, Databases, Genetic, Genome, Software

Abstract

Background: Eukaryotic DNA replication is regulated at the level of large chromosomal domains (0.5-5 megabases in mammals) within which replicons are activated relatively synchronously. These domains replicate in a specific temporal order during S-phase and our genome-wide analyses of replication timing have demonstrated that this temporal order of domain replication is a stable property of specific cell types., Results: We have developed ReplicationDomain http://www.replicationdomain.org as a web-based database for analysis of genome-wide replication timing maps (replication profiles) from various cell lines and species. This database also provides comparative information of transcriptional expression and is configured to display any genome-wide property (for instance, ChIP-Chip or ChIP-Seq data) via an interactive web interface. Our published microarray data sets are publicly available. Users may graphically display these data sets for a selected genomic region and download the data displayed as text files, or alternatively, download complete genome-wide data sets. Furthermore, we have implemented a user registration system that allows registered users to upload their own data sets. Upon uploading, registered users may choose to: (1) view their data sets privately without sharing; (2) share with other registered users; or (3) make their published or "in press" data sets publicly available, which can fulfill journal and funding agencies' requirements for data sharing., Conclusion: ReplicationDomain is a novel and powerful tool to facilitate the comparative visualization of replication timing in various cell types as well as other genome-wide chromatin features and is considerably faster and more convenient than existing browsers when viewing multi-megabase segments of chromosomes. Furthermore, the data upload function with the option of private viewing or sharing of data sets between registered users should be a valuable resource for the scientific community.

Published

2008

32. Global reorganization of replication domains during embryonic stem cell differentiation.

Author

Hiratani I, Ryba T, Itoh M, Yokochi T, Schwaiger M, Chang CW, Lyou Y, Townes TM, Schübeler D, and Gilbert DM

Subjects

Animals, Cell Cycle physiology, Cell Line, Embryonic Stem Cells physiology, Gene Expression Profiling, In Situ Hybridization, Fluorescence, Male, Mice, Oligonucleotide Array Sequence Analysis, Cell Differentiation physiology, DNA Replication physiology, Embryonic Stem Cells cytology, Transcription, Genetic physiology

Abstract

DNA replication in mammals is regulated via the coordinate firing of clusters of replicons that duplicate megabase-sized chromosome segments at specific times during S-phase. Cytogenetic studies show that these "replicon clusters" coalesce as subchromosomal units that persist through multiple cell generations, but the molecular boundaries of such units have remained elusive. Moreover, the extent to which changes in replication timing occur during differentiation and their relationship to transcription changes has not been rigorously investigated. We have constructed high-resolution replication-timing profiles in mouse embryonic stem cells (mESCs) before and after differentiation to neural precursor cells. We demonstrate that chromosomes can be segmented into multimegabase domains of coordinate replication, which we call "replication domains," separated by transition regions whose replication kinetics are consistent with large originless segments. The molecular boundaries of replication domains are remarkably well conserved between distantly related ESC lines and induced pluripotent stem cells. Unexpectedly, ESC differentiation was accompanied by the consolidation of smaller differentially replicating domains into larger coordinately replicated units whose replication time was more aligned to isochore GC content and the density of LINE-1 transposable elements, but not gene density. Replication-timing changes were coordinated with transcription changes for weak promoters more than strong promoters, and were accompanied by rearrangements in subnuclear position. We conclude that replication profiles are cell-type specific, and changes in these profiles reveal chromosome segments that undergo large changes in organization during differentiation. Moreover, smaller replication domains and a higher density of timing transition regions that interrupt isochore replication timing define a novel characteristic of the pluripotent state.

Published

2008

33. Differentiation-induced replication-timing changes are restricted to AT-rich/long interspersed nuclear element (LINE)-rich isochores.

Author

Hiratani I, Leskovar A, and Gilbert DM

Subjects

Animals, Cell Line, Mice, Point Mutation, Polymerase Chain Reaction, Cell Differentiation, Cell Nucleus genetics, Long Interspersed Nucleotide Elements

Abstract

The replication timing of some genes is developmentally regulated, but the significance of replication timing to cellular differentiation has been difficult to substantiate. Studies have largely been restricted to the comparison of a few genes in established cell lines derived from different tissues, and most of these genes do not change replication timing. Hence, it has not been possible to predict how many or what types of genes might be subject to such control. Here, we have evaluated the replication timing of 54 tissue-specific genes in mouse embryonic stem cells before and after differentiation to neural precursors. Strikingly, genes residing within isochores rich in GC and poor in long interspersed nuclear elements (LINEs) did not change their replication timing, whereas half of genes within isochores rich in AT and long interspersed nuclear elements displayed programmed changes in replication timing that accompanied changes in gene expression. Our results provide direct evidence that differentiation-induced autosomal replication-timing changes are a significant part of mammalian development, provide a means to predict genes subject to such regulation, and suggest that replication timing may be more related to the evolution of metazoan genomes than to gene function or expression pattern.

Published

2004

34. Selective degradation of excess Ldb1 by Rnf12/RLIM confers proper Ldb1 expression levels and Xlim-1/Ldb1 stoichiometry in Xenopus organizer functions.

Author

Hiratani I, Yamamoto N, Mochizuki T, Ohmori SY, and Taira M

Subjects

Amino Acid Sequence, Animals, DNA-Binding Proteins genetics, Gastrula metabolism, LIM-Homeodomain Proteins, Mesoderm metabolism, Molecular Sequence Data, Transcription Factors, Xenopus, DNA-Binding Proteins metabolism, Homeodomain Proteins metabolism, Organizers, Embryonic metabolism, Repressor Proteins metabolism, Xenopus Proteins

Abstract

The Xenopus LIM homeodomain (LIM-HD) protein, Xlim-1, is expressed in the Spemann organizer and cooperates with its positive regulator, Ldb1, to activate organizer gene expression. While this activation is presumably mediated through Xlim-1/Ldb1 tetramer formation, the mechanisms regulating proper Xlim-1/Ldb1 stoichiometry remains largely unknown. We isolated the Xenopus ortholog (XRnf12) of the RING finger protein Rnf12/RLIM and explored its functional interactions with Xlim-1 and Ldb1. Although XRnf12 functions as a E3 ubiquitin ligase for Ldb1 and causes proteasome-dependent degradation of Ldb1, we found that co-expression of a high level of Xlim-1 suppresses Ldb1 degradation by XRnf12. This suppression requires both the LIM domains of Xlim-1 and the LIM interaction domain of Ldb1, suggesting that Ldb1, when bound to Xlim-1, escapes degradation by XRnf12. We further show that a high level of Ldb1 suppresses the organizer activity of Xlim-1/Ldb1, suggesting that excess Ldb1 molecules disturb Xlim-1/Ldb1 stoichiometry. Consistent with this, Ldb1 overexpression in the dorsal marginal zone suppresses expression of several organizer genes including postulated Xlim-1 targets, and importantly, this suppression is rescued by co-expression of XRnf12. These data suggest that XRnf12 confers proper Ldb1 protein levels and Xlim-1/Ldb1 stoichiometry for their functions in the organizer. Together with the similarity in the expression pattern of Ldb1 and XRnf12 throughout early embryogenesis, we propose Rnf12/RLIM as a specific regulator of Ldb1 to ensure its proper interactions with LIM-HD proteins and possibly other Ldb1-interacting proteins in the organizer as well as in other tissues.

Published

2003

35. The Xenopus receptor tyrosine kinase Xror2 modulates morphogenetic movements of the axial mesoderm and neuroectoderm via Wnt signaling.

Author

Hikasa H, Shibata M, Hiratani I, and Taira M

Subjects

Amino Acid Sequence, Animals, Carrier Proteins, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Embryo, Nonmammalian cytology, Embryo, Nonmammalian metabolism, Gastrula metabolism, Gene Expression Regulation, Developmental, Glycoproteins genetics, Head abnormalities, Head embryology, Homeodomain Proteins genetics, Homeodomain Proteins metabolism, LIM Domain Proteins, LIM-Homeodomain Proteins, Molecular Sequence Data, Mutation, Neural Tube Defects genetics, Neural Tube Defects metabolism, Notochord embryology, Proteins genetics, Proteins metabolism, Receptor Tyrosine Kinase-like Orphan Receptors genetics, Receptors, Cell Surface genetics, Sequence Homology, Amino Acid, Signal Transduction, Transcription Factors, Wnt Proteins, Xenopus Proteins genetics, Xenopus laevis metabolism, Ectoderm metabolism, Glycoproteins metabolism, Intercellular Signaling Peptides and Proteins, Mesoderm metabolism, Receptor Tyrosine Kinase-like Orphan Receptors metabolism, Receptors, Cell Surface metabolism, Receptors, G-Protein-Coupled, Xenopus Proteins metabolism, Xenopus laevis embryology

Abstract

The Spemann organizer plays a central role in neural induction, patterning of the neuroectoderm and mesoderm, and morphogenetic movements during early embryogenesis. By seeking genes whose expression is activated by the organizer-specific LIM homeobox gene Xlim-1 in Xenopus animal caps, we isolated the receptor tyrosine kinase Xror2. Xror2 is expressed initially in the dorsal marginal zone, then in the notochord and the neuroectoderm posterior to the midbrain-hindbrain boundary. mRNA injection experiments revealed that overexpression of Xror2 inhibits convergent extension of the dorsal mesoderm and neuroectoderm in whole embryos, as well as the elongation of animal caps treated with activin, whereas it does not appear to affect cell differentiation of neural tissue and notochord. Interestingly, mutant constructs in which the kinase domain was point-mutated or deleted (named Xror2-TM) also inhibited convergent extension, and did not counteract the wild-type, suggesting that the ectodomain of Xror2 per se has activities that may be modulated by the intracellular domain. In relation to Wnt signaling for planar cell polarity, we observed: (1) the Frizzled-like domain in the ectodomain is required for the activity of wild-type Xror2 and Xror2-TM; (2) co-expression of Xror2 with Xwnt11, Xfz7, or both, synergistically inhibits convergent extension in embryos; (3) inhibition of elongation by Xror2 in activin-treated animal caps is reversed by co-expression of a dominant negative form of Cdc42 that has been suggested to mediate the planar cell polarity pathway of Wnt; and (4) the ectodomain of Xror2 interacts with Xwnts in co-immunoprecipitation experiments. These results suggest that Xror2 cooperates with Wnts to regulate convergent extension of the axial mesoderm and neuroectoderm by modulating the planar cell polarity pathway of Wnt.

Published

2002

36. Functional domains of the LIM homeodomain protein Xlim-1 involved in negative regulation, transactivation, and axis formation in Xenopus embryos.

Author

Hiratani I, Mochizuki T, Tochimoto N, and Taira M

Subjects

Amino Acid Sequence, Animals, Animals, Genetically Modified, Conserved Sequence, Genes, Reporter, Glutathione Transferase genetics, Homeodomain Proteins chemistry, Homeodomain Proteins genetics, LIM-Homeodomain Proteins, Luciferases genetics, Molecular Sequence Data, Morphogenesis, Organizers, Embryonic physiology, Recombinant Fusion Proteins biosynthesis, Sequence Alignment, Sequence Homology, Amino Acid, Transcription Factors, Transcription, Genetic, Tyrosine, Xenopus Proteins, Body Patterning, Embryo, Nonmammalian physiology, Gene Expression Regulation, Developmental, Homeodomain Proteins physiology, Transcriptional Activation, Xenopus embryology

Abstract

The Xenopus LIM homeodomain protein Xlim-1 is specifically expressed in the Spemann organizer region and assumed to play a role in the establishment of the body axis as a transcriptional activator. To further elucidate the mechanism underlying the regulation of its transcriptional activity, we focused on the region C-terminal to the homeodomain of Xlim-1 (CT239-403) and divided it into five regions, CCR1-5 (C-terminal conserved regions), based on similarity between Xlim-1 and its paralog, Xlim-5. The role of Xlim-1 CT239-403 in the Spemann organizer was analyzed by assaying the axis-forming ability of a series of CCR-mutated constructs in Xenopus embryos. We show that high doses of Xlim-1 constructs deleted of CCR1 or CCR2 initiate secondary axis formation in the absence of its coactivator Ldb1 (LIM-domain-binding protein 1), suggesting that CCR1 and CCR2 are involved in negative regulation of Xlim-1. In contrast, while Xlim-1 is capable of initiating secondary axis formation at low doses in the presence of Ldb1, deletion of CCR2 (aa 275-295) or substitution of five conserved tyrosines in CCR2 with alanines (CCR2-5YA) abolished the activity. In addition, UAS-GAL4 one-hybrid reporter assays in Xenopus showed that CCR2, but not CCR2-5YA, with its flanking regions (aa 261-315) functions as a transactivation domain when fused to the GAL4 DNA-binding domain. Finally, we show that none of the known transcriptional coactivators tested (CBP, SRC-1, and TIF2) interacts with the Xlim-1 transactivation domain (aa 261-315). Thus, Xlim-1 not only contains a unique tyrosine-rich activation domain but also contains a negative regulatory domain in CT239-403, suggesting a complex regulatory mechanism underlying the transcriptional activity of Xlim-1 in the organizer.

Published

2001