bims-crepig Biomed News
on Chromatin regulation and epigenetics in cell fate and cancer
Issue of 2024‒08‒04
twenty-two papers selected by
Connor Rogerson, University of Cambridge
  1. A replisome-associated histone H3-H4 chaperone required for epigenetic inheritance.
  2. Gapped-kmer sequence modeling robustly identifies regulatory vocabularies and distal enhancers conserved between evolutionarily distant mammals.
  3. Prion-like domain mediated phase separation of ARID1A promotes oncogenic potential of Ewing's sarcoma.
  4. Cell fate decision by a morphogen-transcription factor-chromatin modifier axis.
  5. Mrc1 regulates parental histone segregation and heterochromatin inheritance.
  6. guidedNOMe-seq quantifies chromatin states at single allele resolution for hundreds of custom regions in parallel.
  7. Z-DNA formation in promoters conserved between human and mouse are associated with increased transcription reinitiation rates.
  8. The fork protection complex promotes parental histone recycling and epigenetic memory.
  9. STAG2 mutations reshape the cohesin-structured spatial chromatin architecture to drive gene regulation in acute myeloid leukemia.
  10. Enhancer-driven gene regulatory networks inference from single-cell RNA-seq and ATAC-seq data.
  11. Quantifying genome-wide transcription factor binding affinities for chromatin using BANC-seq.
  12. ERK signalling eliminates Nanog and maintains Oct4 to drive the formative pluripotency transition.
  13. mTORC2-driven chromatin cGAS mediates chemoresistance through epigenetic reprogramming in colorectal cancer.
  14. Chrom-seq identifies RNAs at chromatin marks.
  15. Baf155 controls hematopoietic differentiation and regeneration through chromatin priming.
  16. Exploring the roles of RNAs in chromatin architecture using deep learning.
  17. Enhancers associated with unstable RNAs are rare in plants.
  18. Genomic background sequences systematically outperform synthetic ones in de novo motif discovery for ChIP-seq data.
  19. Engineered transcription activator-like effector dimer proteins confer DNA loop-dependent gene repression comparable to Lac repressor.
  20. scaDA: A novel statistical method for differential analysis of single-cell chromatin accessibility sequencing data.
  21. P300 regulates histone crotonylation and preimplantation embryo development.
  22. Gene body DNA hydroxymethylation restricts the magnitude of transcriptional changes during aging.
  1. Cell. 2024 Jul 25. pii: S0092-8674(24)00766-9. [Epub ahead of print]
    A replisome-associated histone H3-H4 chaperone required for epigenetic inheritance.
    Juntao Yu, Yujie Zhang, Yimeng Fang, Joao A Paulo, Dadmehr Yaghoubi, Xu Hua, Gergana Shipkovenska, Takenori Toda, Zhiguo Zhang, Steven P Gygi, Songtao Jia, Qing Li, Danesh Moazed.
      Faithful transfer of parental histones to newly replicated daughter DNA strands is critical for inheritance of epigenetic states. Although replication proteins that facilitate parental histone transfer have been identified, how intact histone H3-H4 tetramers travel from the front to the back of the replication fork remains unknown. Here, we use AlphaFold-Multimer structural predictions combined with biochemical and genetic approaches to identify the Mrc1/CLASPIN subunit of the replisome as a histone chaperone. Mrc1 contains a conserved histone-binding domain that forms a brace around the H3-H4 tetramer mimicking nucleosomal DNA and H2A-H2B histones, is required for heterochromatin inheritance, and promotes parental histone recycling during replication. We further identify binding sites for the FACT histone chaperone in Swi1/TIMELESS and DNA polymerase α that are required for heterochromatin inheritance. We propose that Mrc1, in concert with FACT acting as a mobile co-chaperone, coordinates the distribution of parental histones to newly replicated DNA.
    Keywords:  CLASPIN; FACT; chromatin replication; epigenetics; fork protection complex; heterochromatin; histone inheritance; parental histone transfer; replisome, Mrc1
    DOI:  https://doi.org/10.1016/j.cell.2024.07.006
  2. Nat Commun. 2024 Jul 31. 15(1): 6464
    Gapped-kmer sequence modeling robustly identifies regulatory vocabularies and distal enhancers conserved between evolutionarily distant mammals.
    Jin Woo Oh, Michael A Beer.
      Gene regulatory elements drive complex biological phenomena and their mutations are associated with common human diseases. The impacts of human regulatory variants are often tested using model organisms such as mice. However, mapping human enhancers to conserved elements in mice remains a challenge, due to both rapid enhancer evolution and limitations of current computational methods. We analyze distal enhancers across 45 matched human/mouse cell/tissue pairs from a comprehensive dataset of DNase-seq experiments, and show that while cell-specific regulatory vocabulary is conserved, enhancers evolve more rapidly than promoters and CTCF binding sites. Enhancer conservation rates vary across cell types, in part explainable by tissue specific transposable element activity. We present an improved genome alignment algorithm using gapped-kmer features, called gkm-align, and make genome wide predictions for 1,401,803 orthologous regulatory elements. We show that gkm-align discovers 23,660 novel human/mouse conserved enhancers missed by previous algorithms, with strong evidence of conserved functional activity.
    DOI:  https://doi.org/10.1038/s41467-024-50708-z
  3. Nat Commun. 2024 Aug 03. 15(1): 6569
    Prion-like domain mediated phase separation of ARID1A promotes oncogenic potential of Ewing's sarcoma.
    Yong Ryoul Kim, Jaegeon Joo, Hee Jung Lee, Chaelim Kim, Ju-Chan Park, Young Suk Yu, Chang Rok Kim, Do Hui Lee, Joowon Cha, Hyemin Kwon, Kimberley M Hanssen, Thomas G P Grünewald, Murim Choi, Ilkyu Han, Sangsu Bae, Inkyung Jung, Yongdae Shin, Sung Hee Baek.
      Liquid-liquid phase separation (LLPS) facilitates the formation of membraneless organelles within cells, with implications in various biological processes and disease states. AT-rich interactive domain-containing protein 1A (ARID1A) is a chromatin remodeling factor frequently associated with cancer mutations, yet its functional mechanism remains largely unknown. Here, we find that ARID1A harbors a prion-like domain (PrLD), which facilitates the formation of liquid condensates through PrLD-mediated LLPS. The nuclear condensates formed by ARID1A LLPS are significantly elevated in Ewing's sarcoma patient specimen. Disruption of ARID1A LLPS results in diminished proliferative and invasive abilities in Ewing's sarcoma cells. Through genome-wide chromatin structure and transcription profiling, we identify that the ARID1A condensate localizes to EWS/FLI1 target enhancers and induces long-range chromatin architectural changes by forming functional chromatin remodeling hubs at oncogenic target genes. Collectively, our findings demonstrate that ARID1A promotes oncogenic potential through PrLD-mediated LLPS, offering a potential therapeutic approach for treating Ewing's sarcoma.
    DOI:  https://doi.org/10.1038/s41467-024-51050-0
  4. Nat Commun. 2024 Jul 29. 15(1): 6365
    Cell fate decision by a morphogen-transcription factor-chromatin modifier axis.
    Jin Ming, Lihui Lin, Jiajun Li, Linlin Wu, Shicai Fang, Tao Huang, Yu Fu, Dong Liu, Wenhui Zhang, Chen Li, Yongzheng Yang, Yi Huang, Yue Qin, Junqi Kuang, Xingnan Huang, Liman Guo, Xiaofei Zhang, Jing Liu, Jiekai Chen, Chengchen Zhao, Bo Wang, Duanqing Pei.
      Cell fate decisions remain poorly understood at the molecular level. Embryogenesis provides a unique opportunity to analyze molecular details associated with cell fate decisions. Works based on model organisms have provided a conceptual framework of genes that specify cell fate control, for example, transcription factors (TFs) controlling processes from pluripotency to immunity1. How TFs specify cell fate remains poorly understood. Here we report that SALL4 relies on NuRD (nucleosome-remodeling and deacetylase complex) to interpret BMP4 signal and decide cell fate in a well-controlled in vitro system. While NuRD complex cooperates with SALL4 to convert mouse embryonic fibroblasts or MEFs to pluripotency, BMP4 diverts the same process to an alternative fate, PrE (primitive endoderm). Mechanistically, BMP4 signals the dissociation of SALL4 from NuRD physically to establish a gene regulatory network for PrE. Our results provide a conceptual framework to explore the rich landscapes of cell fate choices intrinsic to development in higher organisms involving morphogen-TF-chromatin modifier pathways.
    DOI:  https://doi.org/10.1038/s41467-024-50144-z
  5. Mol Cell. 2024 Jul 23. pii: S1097-2765(24)00573-2. [Epub ahead of print]
    Mrc1 regulates parental histone segregation and heterochromatin inheritance.
    Takenori Toda, Yimeng Fang, Chun-Min Shan, Xu Hua, Jin-Kwang Kim, Lauren Clarissa Tang, Marko Jovanovic, Liang Tong, Feng Qiao, Zhiguo Zhang, Songtao Jia.
      Chromatin-based epigenetic memory relies on the symmetric distribution of parental histones to newly synthesized daughter DNA strands, aided by histone chaperones within the DNA replication machinery. However, the mechanism of parental histone transfer remains elusive. Here, we reveal that in fission yeast, the replisome protein Mrc1 plays a crucial role in promoting the transfer of parental histone H3-H4 to the lagging strand, ensuring proper heterochromatin inheritance. In addition, Mrc1 facilitates the interaction between Mcm2 and DNA polymerase alpha, two histone-binding proteins critical for parental histone transfer. Furthermore, Mrc1's involvement in parental histone transfer and epigenetic inheritance is independent of its known functions in DNA replication checkpoint activation and replisome speed control. Instead, Mrc1 interacts with Mcm2 outside of its histone-binding region, creating a physical barrier to separate parental histone transfer pathways. These findings unveil Mrc1 as a key player within the replisome, coordinating parental histone segregation to regulate epigenetic inheritance.
    Keywords:  H3K9 methylation; Mcm2; Mrc1; Swi7; epigenetic inheritance; heterochromatin; histone
    DOI:  https://doi.org/10.1016/j.molcel.2024.07.002
  6. BMC Genomics. 2024 Jul 29. 25(1): 732
    guidedNOMe-seq quantifies chromatin states at single allele resolution for hundreds of custom regions in parallel.
    Michaela Schwaiger, Fabio Mohn, Marc Bühler, Lucas J T Kaaij.
      Since the introduction of next generation sequencing technologies, the field of epigenomics has evolved rapidly. However, most commonly used assays are enrichment-based methods and thus only semi-quantitative. Nucleosome occupancy and methylome sequencing (NOMe-seq) allows for quantitative inference of chromatin states with single locus resolution, but this requires high sequencing depth and is therefore prohibitively expensive to routinely apply to organisms with large genomes. To overcome this limitation, we introduce guidedNOMe-seq, where we combine NOMe profiling with large scale sgRNA synthesis and Cas9-mediated region-of-interest (ROI) liberation. To facilitate quantitative comparisons between multiple samples, we additionally develop an R package to standardize differential analysis of any type of NOMe-seq data. We extensively benchmark guidedNOMe-seq in a proof-of-concept study, dissecting the interplay of ChAHP and CTCF on chromatin. In summary we present a cost-effective, scalable, and customizable target enrichment extension to the existing NOMe-seq protocol allowing genome-scale quantification of nucleosome occupancy and transcription factor binding at single allele resolution.
    Keywords:  CTCF; Cas9 enrichment; ChAHP; Chromatin; NOMe-Seq
    DOI:  https://doi.org/10.1186/s12864-024-10625-3
  7. Sci Rep. 2024 Aug 01. 14(1): 17786
    Z-DNA formation in promoters conserved between human and mouse are associated with increased transcription reinitiation rates.
    Nazar Beknazarov, Dmitry Konovalov, Alan Herbert, Maria Poptsova.
      A long-standing question concerns the role of Z-DNA in transcription. Here we use a deep learning approach DeepZ that predicts Z-flipons based on DNA sequence, structural properties of nucleotides and omics data. We examined Z-flipons that are conserved between human and mouse genomes after generating whole-genome Z-flipon maps and then validated them by orthogonal approaches based on high resolution chemical mapping of Z-DNA and the transformer algorithm Z-DNABERT. For human and mouse, we revealed similar pattern of transcription factors, chromatin remodelers, and histone marks associated with conserved Z-flipons. We found significant enrichment of Z-flipons in alternative and bidirectional promoters associated with neurogenesis genes. We show that conserved Z-flipons are associated with increased experimentally determined transcription reinitiation rates compared to promoters without Z-flipons, but without affecting elongation or pausing. Our findings support a model where Z-flipons engage Transcription Factor E and impact phenotype by enabling the reset of preinitiation complexes when active, and the suppression of gene expression when engaged by repressive chromatin complexes.
    DOI:  https://doi.org/10.1038/s41598-024-68439-y
  8. Cell. 2024 Jul 26. pii: S0092-8674(24)00777-3. [Epub ahead of print]
    The fork protection complex promotes parental histone recycling and epigenetic memory.
    Sebastian Jespersen Charlton, Valentin Flury, Yutaka Kanoh, Aitana Victoria Genzor, Leonie Kollenstart, Wantong Ao, Peter Brøgger, Melanie Bianca Weisser, Marek Adamus, Nicolas Alcaraz, Charlotte M Delvaux de Fenffe, Francesca Mattiroli, Guillermo Montoya, Hisao Masai, Anja Groth, Geneviève Thon.
      The inheritance of parental histones across the replication fork is thought to mediate epigenetic memory. Here, we reveal that fission yeast Mrc1 (CLASPIN in humans) binds H3-H4 tetramers and operates as a central coordinator of symmetric parental histone inheritance. Mrc1 mutants in a key connector domain disrupted segregation of parental histones to the lagging strand comparable to Mcm2 histone-binding mutants. Both mutants showed clonal and asymmetric loss of H3K9me-mediated gene silencing. AlphaFold predicted co-chaperoning of H3-H4 tetramers by Mrc1 and Mcm2, with the Mrc1 connector domain bridging histone and Mcm2 binding. Biochemical and functional analysis validated this model and revealed a duality in Mrc1 function: disabling histone binding in the connector domain disrupted lagging-strand recycling while another histone-binding mutation impaired leading strand recycling. We propose that Mrc1 toggles histones between the lagging and leading strand recycling pathways, in part by intra-replisome co-chaperoning, to ensure epigenetic transmission to both daughter cells.
    Keywords:  Claspin; DNA replication; H3K9 methylation; chromatin replication; epigenetic inheritance; epigenome maintenance; fission yeast; heterochromatin; histone chaperone; histone recycling; mouse embryonic stem cells
    DOI:  https://doi.org/10.1016/j.cell.2024.07.017
  9. Cell Rep. 2024 Jul 25. pii: S2211-1247(24)00827-1. [Epub ahead of print] 114498
    STAG2 mutations reshape the cohesin-structured spatial chromatin architecture to drive gene regulation in acute myeloid leukemia.
    Alexander Fischer, Benjamín Hernández-Rodríguez, Roger Mulet-Lazaro, Margit Nuetzel, Fabian Hölzl, Stanley van Herk, François G Kavelaars, Hanna Stanewsky, Ute Ackermann, Amadou H Niang, Noelia Diaz, Edith Reuschel, Nicholas Strieder, Inmaculada Hernández-López, Peter J M Valk, Juan M Vaquerizas, Michael Rehli, Ruud Delwel, Claudia Gebhard.
      Cohesin shapes the chromatin architecture, including enhancer-promoter interactions. Its components, especially STAG2, but not its paralog STAG1, are frequently mutated in myeloid malignancies. To elucidate the underlying mechanisms of leukemogenesis, we comprehensively characterized genetic, transcriptional, and chromatin conformational changes in acute myeloid leukemia (AML) patient samples. Specific loci displayed altered cohesin occupancy, gene expression, and local chromatin activation, which were not compensated by the remaining STAG1-cohesin. These changes could be linked to disrupted spatial chromatin looping in cohesin-mutated AMLs. Complementary depletion of STAG2 or STAG1 in primary human hematopoietic progenitors (HSPCs) revealed effects resembling STAG2-mutant AML-specific changes following STAG2 knockdown, not invoked by the depletion of STAG1. STAG2-deficient HSPCs displayed impaired differentiation capacity and maintained HSPC-like gene expression. This work establishes STAG2 as a key regulator of chromatin contacts, gene expression, and differentiation in the hematopoietic system and identifies candidate target genes that may be implicated in human leukemogenesis.
    Keywords:  CP: Cancer; CP: Molecular biology; Hi-C; RAD21; STAG2; acute myeloid leukemia; cohesin mutations; epigenetics; gene regulation; hematopoiesis; hematopoietic stem and progenitor cells; spatial chromatin structure
    DOI:  https://doi.org/10.1016/j.celrep.2024.114498
  10. Brief Bioinform. 2024 Jul 25. pii: bbae369. [Epub ahead of print]25(5):
    Enhancer-driven gene regulatory networks inference from single-cell RNA-seq and ATAC-seq data.
    Yang Li, Anjun Ma, Yizhong Wang, Qi Guo, Cankun Wang, Hongjun Fu, Bingqiang Liu, Qin Ma.
      Deciphering the intricate relationships between transcription factors (TFs), enhancers, and genes through the inference of enhancer-driven gene regulatory networks (eGRNs) is crucial in understanding gene regulatory programs in a complex biological system. This study introduces STREAM, a novel method that leverages a Steiner forest problem model, a hybrid biclustering pipeline, and submodular optimization to infer eGRNs from jointly profiled single-cell transcriptome and chromatin accessibility data. Compared to existing methods, STREAM demonstrates enhanced performance in terms of TF recovery, TF-enhancer linkage prediction, and enhancer-gene relation discovery. Application of STREAM to an Alzheimer's disease dataset and a diffuse small lymphocytic lymphoma dataset reveals its ability to identify TF-enhancer-gene relations associated with pseudotime, as well as key TF-enhancer-gene relations and TF cooperation underlying tumor cells.
    Keywords:  Steiner forest problem model; biological network; data integration; scATAC-seq; scRNA-seq; submodular optimization
    DOI:  https://doi.org/10.1093/bib/bbae369
  11. Nat Protoc. 2024 Jul 30.
    Quantifying genome-wide transcription factor binding affinities for chromatin using BANC-seq.
    Roelof A Wester, Hannah K Neikes, Rik G H Lindeboom, Michiel Vermeulen.
      Transcription factors (TFs) bind specific DNA sequences to regulate transcription. Apart from DNA sequences, local factors such as DNA accessibility and chromatin structure determine the affinity of a TF for any given locus. Including these factors when measuring TF-DNA affinities has proven difficult. To address this challenge, we recently developed a method called binding affinities in native chromatin by sequencing (BANC-seq). In BANC-seq, intact mammalian nuclei are incubated with a concentration range of epitope-tagged TF, followed by either chromatin immunoprecipitation or cleavage under target and release using nuclease with spike-in DNA. This allows determination of apparent dissociation constant (KdApp) values, defined by the concentration of TF at which half-maximum binding occurs, across the genome. Here we present a detailed stepwise protocol for BANC-seq, including downstream data analysis. In principle, any molecular biologist should be able to perform a BANC-seq experiment in as little as 1.5 d (excluding analysis). However, preprocessing and analysis of the sequencing data does require some experience in command-line shell and R programming.
    DOI:  https://doi.org/10.1038/s41596-024-01026-7
  12. Development. 2024 Jul 15. pii: dev203106. [Epub ahead of print]151(14):
    ERK signalling eliminates Nanog and maintains Oct4 to drive the formative pluripotency transition.
    Carla Mulas, Melanie Stammers, Siiri I Salomaa, Constanze Heinzen, David M Suter, Austin Smith, Kevin J Chalut.
      Naïve epiblast cells in the embryo and pluripotent stem cells in vitro undergo developmental progression to a formative state competent for lineage specification. During this transition, transcription factors and chromatin are rewired to encode new functional features. Here, we examine the role of mitogen-activated protein kinase (ERK1/2) signalling in pluripotent state transition. We show that a primary consequence of ERK activation in mouse embryonic stem cells is elimination of Nanog, which precipitates breakdown of the naïve state gene regulatory network. Variability in pERK dynamics results in heterogeneous loss of Nanog and metachronous state transition. Knockdown of Nanog allows exit without ERK activation. However, transition to formative pluripotency does not proceed and cells collapse to an indeterminate identity. This outcome is due to failure to maintain expression of the central pluripotency factor Oct4. Thus, during formative transition ERK signalling both dismantles the naïve state and preserves pluripotency. These results illustrate how a single signalling pathway can both initiate and secure transition between cell states.
    Keywords:  Differentiation; ERK; Formative; Mouse embryonic stem cells; Naive; Nanog
    DOI:  https://doi.org/10.1242/dev.203106
  13. Nat Cell Biol. 2024 Jul 30.
    mTORC2-driven chromatin cGAS mediates chemoresistance through epigenetic reprogramming in colorectal cancer.
    Guoqing Lv, Qian Wang, Lin Lin, Qiao Ye, Xi Li, Qian Zhou, Xiangzhen Kong, Hongxia Deng, Fuping You, Hebing Chen, Song Wu, Lin Yuan.
      Cyclic GMP-AMP synthase (cGAS), a cytosolic DNA sensor that initiates a STING-dependent innate immune response, binds tightly to chromatin, where its catalytic activity is inhibited; however, mechanisms underlying cGAS recruitment to chromatin and functions of chromatin-bound cGAS (ccGAS) remain unclear. Here we show that mTORC2-mediated phosphorylation of human cGAS serine 37 promotes its chromatin localization in colorectal cancer cells, regulating cell growth and drug resistance independently of STING. We discovered that ccGAS recruits the SWI/SNF complex at specific chromatin regions, modifying expression of genes linked to glutaminolysis and DNA replication. Although ccGAS depletion inhibited cell growth, it induced chemoresistance to fluorouracil treatment in vitro and in vivo. Moreover, blocking kidney-type glutaminase, a downstream ccGAS target, overcame chemoresistance caused by ccGAS loss. Thus, ccGAS coordinates colorectal cancer plasticity and acquired chemoresistance through epigenetic patterning. Targeting both mTORC2-ccGAS and glutaminase provides a promising strategy to eliminate quiescent resistant cancer cells.
    DOI:  https://doi.org/10.1038/s41556-024-01473-0
  14. Sci Adv. 2024 Aug 02. 10(31): eadn1397
    Chrom-seq identifies RNAs at chromatin marks.
    Ligang Fan, Wei Sun, Yitong Lyu, Furong Ju, Wenju Sun, Jie Chen, Haiqian Ma, Shifei Yang, Xiaomin Zhou, Nan Wu, Wenkai Yi, Erfei Chen, Rodrigo Villaseñor, Tuncay Baubec, Jian Yan.
      Chromatin marks are associated with transcriptional regulatory activities. However, very few lncRNAs have been characterized with the role in regulating epigenetic marks, largely due to the technical difficulty in identifying chromatin-associating RNA. Current methods are largely limited by the availability of ChIP-grade antibody and the crosslinking, which generates high noise. Here, we developed a method termed Chrom-seq to efficiently capture RNAs associated with various chromatin marks in living cells. Chrom-seq jointly applies highly specific chromatin mark reader with APEX2, which catalyzes the oxidation of biotin-aniline to label the adjacent RNAs for isolation by streptavidin-coated beads. Using the readers of mCBX7/dPC, mCBX1, and mTAF3, we detected RNA species significantly associated with H3K27me3, H3K9me3, and H3K4me3, respectively. We demonstrated that Chrom-seq outperformed other equivalent methods in terms of sensitivity, efficiency, and cost of practice. It provides an antibody-free approach to systematically map RNAs at chromatin marks with potential regulatory roles in epigenetic events.
    DOI:  https://doi.org/10.1126/sciadv.adn1397
  15. Cell Rep. 2024 Jul 30. pii: S2211-1247(24)00887-8. [Epub ahead of print]43(8): 114558
    Baf155 controls hematopoietic differentiation and regeneration through chromatin priming.
    Jun Wu, Changxu Fan, Ashraf Ul Kabir, Karen Krchma, Minseo Kim, Yoojung Kwon, Xiaoyun Xing, Ting Wang, Kyunghee Choi.
      Chromatin priming promotes cell-type-specific gene expression, lineage differentiation, and development. The mechanism of chromatin priming has not been fully understood. Here, we report that mouse hematopoietic stem and progenitor cells (HSPCs) lacking the Baf155 subunit of the BAF (BRG1/BRM-associated factor) chromatin remodeling complex produce a significantly reduced number of mature blood cells, leading to a failure of hematopoietic regeneration upon transplantation and 5-fluorouracil (5-FU) injury. Baf155-deficient HSPCs generate particularly fewer neutrophils, B cells, and CD8+ T cells at homeostasis, supporting a more immune-suppressive tumor microenvironment and enhanced tumor growth. Single-nucleus multiomics analysis reveals that Baf155-deficient HSPCs fail to establish accessible chromatin in selected regions that are enriched for putative enhancers and binding motifs of hematopoietic lineage transcription factors. Our study provides a fundamental mechanistic understanding of the role of Baf155 in hematopoietic lineage chromatin priming and the functional consequences of Baf155 deficiency in regeneration and tumor immunity.
    Keywords:  Baf155; CP: Molecular biology; CP: Stem cell research; Smarcc1; Srg3; chromatin priming; hematopoietic lineage differentiation; hematopoietic regeneration; hematopoietic stem cell; tumor immunity
    DOI:  https://doi.org/10.1016/j.celrep.2024.114558
  16. Nat Commun. 2024 Jul 29. 15(1): 6373
    Exploring the roles of RNAs in chromatin architecture using deep learning.
    Shuzhen Kuang, Katherine S Pollard.
      Recent studies have highlighted the impact of both transcription and transcripts on 3D genome organization, particularly its dynamics. Here, we propose a deep learning framework, called AkitaR, that leverages both genome sequences and genome-wide RNA-DNA interactions to investigate the roles of chromatin-associated RNAs (caRNAs) on genome folding in HFFc6 cells. In order to disentangle the cis- and trans-regulatory roles of caRNAs, we have compared models with nascent transcripts, trans-located caRNAs, open chromatin data, or DNA sequence alone. Both nascent transcripts and trans-located caRNAs improve the models' predictions, especially at cell-type-specific genomic regions. Analyses of feature importance scores reveal the contribution of caRNAs at TAD boundaries, chromatin loops and nuclear sub-structures such as nuclear speckles and nucleoli to the models' predictions. Furthermore, we identify non-coding RNAs (ncRNAs) known to regulate chromatin structures, such as MALAT1 and NEAT1, as well as several new RNAs, RNY5, RPPH1, POLG-DT and THBS1-IT1, that might modulate chromatin architecture through trans-interactions in HFFc6. Our modeling also suggests that transcripts from Alus and other repetitive elements may facilitate chromatin interactions through trans R-loop formation. Our findings provide insights and generate testable hypotheses about the roles of caRNAs in shaping chromatin organization.
    DOI:  https://doi.org/10.1038/s41467-024-50573-w
  17. Nat Plants. 2024 Jul 30.
    Enhancers associated with unstable RNAs are rare in plants.
    Bayley R McDonald, Colette L Picard, Ian M Brabb, Marina I Savenkova, Robert J Schmitz, Steven E Jacobsen, Sascha H Duttke.
      Unstable transcripts have emerged as markers of active enhancers in vertebrates and shown to be involved in many cellular processes and medical disorders. However, their prevalence and role in plants is largely unexplored. Here, we comprehensively captured all actively initiating (nascent) transcripts across diverse crops and other plants using capped small (cs)RNA sequencing. We discovered that unstable transcripts are rare in plants, unlike in vertebrates, and when present, often originate from promoters. In addition, many 'distal' elements in plants initiate tissue-specific stable transcripts and are likely bona fide promoters of as-yet-unannotated genes or non-coding RNAs, cautioning against using reference genome annotations to infer putative enhancer sites. To investigate enhancer function, we integrated data from self-transcribing active regulatory region (STARR) sequencing. We found that annotated promoters and other regions that initiate stable transcripts, but not those marked by unstable or bidirectional unstable transcripts, showed stronger enhancer activity in this assay. Our findings underscore the blurred line between promoters and enhancers and suggest that cis-regulatory elements can encompass diverse structures and mechanisms in eukaryotes, including humans.
    DOI:  https://doi.org/10.1038/s41477-024-01741-9
  18. NAR Genom Bioinform. 2024 Sep;6(3): lqae090
    Genomic background sequences systematically outperform synthetic ones in de novo motif discovery for ChIP-seq data.
    Vladimir V Raditsa, Anton V Tsukanov, Anton G Bogomolov, Victor G Levitsky.
      Efficient de novo motif discovery from the results of wide-genome mapping of transcription factor binding sites (ChIP-seq) is dependent on the choice of background nucleotide sequences. The foreground sequences (ChIP-seq peaks) represent not only specific motifs of target transcription factors, but also the motifs overrepresented throughout the genome, such as simple sequence repeats. We performed a massive comparison of the 'synthetic' and 'genomic' approaches to generate background sequences for de novo motif discovery. The 'synthetic' approach shuffled nucleotides in peaks, while in the 'genomic' approach selected sequences from the reference genome randomly or only from gene promoters according to the fraction of A/T nucleotides in each sequence. We compiled the benchmark collections of ChIP-seq datasets for mouse, human and Arabidopsis, and performed de novo motif discovery. We showed that the genomic approach has both more robust detection of the known motifs of target transcription factors and more stringent exclusion of the simple sequence repeats as possible non-specific motifs. The advantage of the genomic approach over the synthetic approach was greater in plants compared to mammals. We developed the AntiNoise web service (https://denovosea.icgbio.ru/antinoise/) that implements a genomic approach to extract genomic background sequences for twelve eukaryotic genomes.
    DOI:  https://doi.org/10.1093/nargab/lqae090
  19. Nucleic Acids Res. 2024 Jul 30. pii: gkae656. [Epub ahead of print]
    Engineered transcription activator-like effector dimer proteins confer DNA loop-dependent gene repression comparable to Lac repressor.
    Nicole A Becker, Justin P Peters, Elizabeth Lewis, Camden L Daby, Karl Clark, L James Maher.
      Natural prokaryotic gene repression systems often exploit DNA looping to increase the local concentration of gene repressor proteins at a regulated promoter via contributions from repressor proteins bound at distant sites. Using principles from the Escherichia coli lac operon we design analogous repression systems based on target sequence-programmable Transcription Activator-Like Effector dimer (TALED) proteins. Such engineered switches may be valuable for synthetic biology and therapeutic applications. Previous TALEDs with inducible non-covalent dimerization showed detectable, but limited, DNA loop-based repression due to the repressor protein dimerization equilibrium. Here, we show robust DNA loop-dependent bacterial promoter repression by covalent TALEDs and verify that DNA looping dramatically enhances promoter repression in E. coli. We characterize repression using a thermodynamic model that quantitates this favorable contribution of DNA looping. This analysis unequivocally and quantitatively demonstrates that optimized TALED proteins can drive loop-dependent promoter repression in E. coli comparable to the natural LacI repressor system. This work elucidates key design principles that set the stage for wide application of TALED-dependent DNA loop-based repression of target genes.
    DOI:  https://doi.org/10.1093/nar/gkae656
  20. PLoS Comput Biol. 2024 Aug 02. 20(8): e1011854
    scaDA: A novel statistical method for differential analysis of single-cell chromatin accessibility sequencing data.
    Fengdi Zhao, Xin Ma, Bing Yao, Qing Lu, Li Chen.
      Single-cell ATAC-seq sequencing data (scATAC-seq) has been widely used to investigate chromatin accessibility on the single-cell level. One important application of scATAC-seq data analysis is differential chromatin accessibility (DA) analysis. However, the data characteristics of scATAC-seq such as excessive zeros and large variability of chromatin accessibility across cells impose a unique challenge for DA analysis. Existing statistical methods focus on detecting the mean difference of the chromatin accessible regions while overlooking the distribution difference. Motivated by real data exploration that distribution difference exists among cell types, we introduce a novel composite statistical test named "scaDA", which is based on zero-inflated negative binomial model (ZINB), for performing differential distribution analysis of chromatin accessibility by jointly testing the abundance, prevalence and dispersion simultaneously. Benefiting from both dispersion shrinkage and iterative refinement of mean and prevalence parameter estimates, scaDA demonstrates its superiority to both ZINB-based likelihood ratio tests and published methods by achieving the highest power and best FDR control in a comprehensive simulation study. In addition to demonstrating the highest power in three real sc-multiome data analyses, scaDA successfully identifies differentially accessible regions in microglia from sc-multiome data for an Alzheimer's disease (AD) study that are most enriched in GO terms related to neurogenesis and the clinical phenotype of AD, and AD-associated GWAS SNPs.
    DOI:  https://doi.org/10.1371/journal.pcbi.1011854
  21. Nat Commun. 2024 Jul 30. 15(1): 6418
    P300 regulates histone crotonylation and preimplantation embryo development.
    Di Gao, Chao Li, Shao-Yuan Liu, Teng-Teng Xu, Xiao-Ting Lin, Yong-Peng Tan, Fu-Min Gao, Li-Tao Yi, Jian V Zhang, Jun-Yu Ma, Tie-Gang Meng, William S B Yeung, Kui Liu, Xiang-Hong Ou, Rui-Bao Su, Qing-Yuan Sun.
      Histone lysine crotonylation, an evolutionarily conserved modification differing from acetylation, exerts pivotal control over diverse biological processes. Among these are gene transcriptional regulation, spermatogenesis, and cell cycle processes. However, the dynamic changes and functions of histone crotonylation in preimplantation embryonic development in mammals remain unclear. Here, we show that the transcription coactivator P300 functions as a writer of histone crotonylation during embryonic development. Depletion of P300 results in significant developmental defects and dysregulation of the transcriptome of embryos. Importantly, we demonstrate that P300 catalyzes the crotonylation of histone, directly stimulating transcription and regulating gene expression, thereby ensuring successful progression of embryo development up to the blastocyst stage. Moreover, the modification of histone H3 lysine 18 crotonylation (H3K18cr) is primarily localized to active promoter regions. This modification serves as a distinctive epigenetic indicator of crucial transcriptional regulators, facilitating the activation of gene transcription. Together, our results propose a model wherein P300-mediated histone crotonylation plays a crucial role in regulating the fate of embryonic development.
    DOI:  https://doi.org/10.1038/s41467-024-50731-0
  22. Nat Commun. 2024 Jul 28. 15(1): 6357
    Gene body DNA hydroxymethylation restricts the magnitude of transcriptional changes during aging.
    James R Occean, Na Yang, Yan Sun, Marshall S Dawkins, Rachel Munk, Cedric Belair, Showkat Dar, Carlos Anerillas, Lin Wang, Changyou Shi, Christopher Dunn, Michel Bernier, Nathan L Price, Julie S Kim, Chang-Yi Cui, Jinshui Fan, Moitrayee Bhattacharyya, Supriyo De, Manolis Maragkakis, Rafael de Cabo, Simone Sidoli, Payel Sen.
      DNA hydroxymethylation (5hmC), the most abundant oxidative derivative of DNA methylation, is typically enriched at enhancers and gene bodies of transcriptionally active and tissue-specific genes. Although aberrant genomic 5hmC has been implicated in age-related diseases, its functional role in aging remains unknown. Here, using mouse liver and cerebellum as model organs, we show that 5hmC accumulates in gene bodies associated with tissue-specific function and restricts the magnitude of gene expression changes with age. Mechanistically, 5hmC decreases the binding of splicing associated factors and correlates with age-related alternative splicing events. We found that various age-related contexts, such as prolonged quiescence and senescence, drive the accumulation of 5hmC with age. We provide evidence that this age-related transcriptionally restrictive function is conserved in mouse and human tissues. Our findings reveal that 5hmC regulates tissue-specific function and may play a role in longevity.
    DOI:  https://doi.org/10.1038/s41467-024-50725-y
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