User:Khadem.mahdi/Topologically associating domain

From Wikipedia, the free encyclopedia
Topologically associating domains within chromosome territories, their borders and interactions


Topologically associating domains within chromosome territories, their borders and interactions

A topologically associating domain (TAD) is a self-interacting genomic region, meaning that DNA sequences within a TAD physically interact with each other more frequently than with sequences outside the TAD.[1] The median size of TAD in mouse cells is 880 kb which is found to be similar in non-mammalian species.[2] Boundaries at both side of the these domains are conserved between different mammalian cell types and even across species[2] and are highly enriched with CCCTC-binding factor (CTCF) and cohesin binding sites.[1] In addition, some types of genes (such as transfer RNA genes and housekeeping genes) appear near TAD boundaries more often than would be expected by chance.[3][4]

The functions of TADs are not fully understood and still is a matter of debate. Most of the studies indicate TADs regulate gene expression by limiting the enhancer-promoter interaction to each TAD[5], however, recent study uncouples TAD organization and gene expression. [6] Disruption of TAD boundaries are found to be associated with wide range of diseases such as cancer,[7][8][9] variety of limb malformations such as synpolydactyly, Cooks syndrome, and F-syndrome [10], and number of brain disorders like Hypoplastic corpus callosum and Adult-onset demyelinating leukodystrophy[10] .

The mechanisms underlying TAD formation are also complex and not yet fully elucidated, though a number of protein complexes and DNA elements are associated with TAD boundaries. However, the handcuff model and the loop extrusion model are described to describe the TAD formation by the aid of CTCF and cohesin proteins.[11] Furthermore, it has been proposed that the stiffness of TAD boundaries itself could cause the domain insulation and TAD formation.[11]

Discovery and Diversity[edit]

TADs are defined as regions whose DNA sequences preferentially contact each other. They were discovered in 2012 using chromosome conformation capture techniques including Hi-C.[3][12][4] They have been shown to be present in multiple species[13], including fruit flies (Drosophila),[14] mouse[3],plants, fungi and human[4] genomes in bacteria, they are referred to as Chromosomal Interacting Domains (CIDs).[13]

Analytical tools and Databases[edit]

TAD locations are defined by applying an algorithm to Hi-C data. For example, TADs are often called according to the so-called "directionality index".[4] The directionality index is calculated for individual 40kb bins, by collecting the reads that fall in the bin, and observing whether their paired reads map upstream or downstream of the bin (read pairs are required to span no more than 2Mb). A positive value indicates that more read pairs lie downstream than upstream, and a negative value indicates the reverse. Mathematically, the directionality index is a signed chi-square statistic.

The development of 3D genome browsers and databases such as The 3D Genome Browser[15], 3DIV[16], and 3D-GNOME[17] have enabled us to visualize the TAD organization of regions of interest in different cell types.

Mechanisms of formation[edit]

DNA loop extrusion through cohesin rings

A number of proteins are known to be associated with TAD formation including the protein CTCF and the protein complex cohesin.[1] It is also unknown what components are required at TAD boundaries; however, in mammalian cells, it has been shown that these boundary regions have comparatively high levels of CTCF binding.

Computer simulations have shown that chromatin loop extrusion driven by transcription generated supercoiling ensures that cohesin relocalizes quickly and loops grow with reasonable speed and in a good direction. In addition, the supercoiling-driven loop extrusion mechanism is consistent with earlier explanations proposing why TADs flanked by convergent CTCF binding sites form more stable chromatin loops than TADs flanked by divergent CTCF binding sites. In this model, the supercoiling also stimulates enhancer promoter contacts and it is proposed that transcription of eRNA sends the first wave of supercoiling that can activate mRNA transcription in a given TAD.[18][19] Computational models also showed that cohesin rings act like a very efficient molecular comb, pushing knots and entanglements such as in catenanes towards border of TADs where these are removed by the action of topoisomerases. Consistently, removal of entanglements during loop extrusion also increases degree of segregation between chromosomes.[20] However, proof for DNA loop-extrusion is so far limited to condensin (cohesin's sister protein complex) only.[21]

Properties[edit]

Conservation[edit]

TADs have been reported to be relatively constant between different cell types (in stem cells and blood cells, for example), and even between species in specific cases.[22]

Relationship with promoter-enhancer contacts[edit]

The majority of observed interactions between promoters and enhancers do not cross TAD boundaries. Removing a TAD boundary (for example, using CRISPR to delete the relevant region of the genome) can allow new promoter-enhancer contacts to form. This can affect gene expression nearby - such misregulation has been shown to cause limb malformations (e.g. polydactyly) in humans and mice.[22]

Computer simulations have shown that transcription-induced supercoiling of chromatin fibres can explain how TADs are formed and how they can assure very efficient interactions between enhancers and their cognate promoters located in the same TAD.[19]

Relationship with other structural features of the genome[edit]

TADs have been reported to be the same as replication domains, regions of the genome that are copied (replicated) at the same time during S phase of cell division.[23] Insulated neighborhoods, DNA loops formed by CTCF/cohesin-bound regions, are proposed to functionally underlie TADs.[24]

Role in disease[edit]

Disruption of TAD boundaries can affect the expression of nearby genes, and this can cause disease.[25]

For example, genomic structural variants that disrupt TAD boundaries have been reported to cause developmental disorders such as human limb malformations.[26][27][28] Additionally, several studies have provided evidence that the disruption or rearrangement of TAD boundaries can provide growth advantages to certain cancers, such as T-cell acute lymphoblastic leukemia (T-ALL),[29] gliomas,[30] and lung cancer.[31]

Lamina-associated domains[edit]

LADs (dark gray lines) and proteins that interact with them. Lamina is indicated by green curve.
Main article: Nuclear lamina

Lamina-associated domains (LADs) are parts of the chromatin that heavily interact with the lamina, a network-like structure at the inner membrane of the nucleus.[32] LADs consist mostly of transcriptionally silent chromatin, being enriched with trimethylated Lys27 on histone H3, which is a common posttranslational histone modification of heterochromatin.[33] LADs have CTCF-binding sites at their periphery.[32]

See also[edit]

References[edit]

  1. ^ a b c Pombo, A; Dillon, N (April 2015). "Three-dimensional genome architecture: players and mechanisms". Nature Reviews Molecular Cell Biology. 16 (4): 245–57. doi:10.1038/nrm3965. PMID 25757416.
  2. ^ a b Yu, Miao; Ren, Bing (2017). "The Three-Dimensional Organization of Mammalian Genomes". Annual Review of Cell and Developmental Biology. 33: 265–289. doi:10.1146/annurev-cellbio-100616-060531. ISSN 1530-8995. PMC 5837811. PMID 28783961.
  3. ^ a b c Nora, Elphège P.; Lajoie, Bryan R.; Schulz, Edda G.; Giorgetti, Luca; Okamoto, Ikuhiro; Servant, Nicolas; Piolot, Tristan; Van Berkum, Nynke L.; Meisig, Johannes; Sedat, John; Gribnau, Joost; Barillot, Emmanuel; Blüthgen, Nils; Dekker, Job; Heard, Edith (2012). "Spatial partitioning of the regulatory landscape of the X-inactivation centre". Nature. 485 (7398): 381–385. Bibcode:2012Natur.485..381N. doi:10.1038/nature11049. PMC 3555144. PMID 22495304.
  4. ^ a b c d Dixon, J. R.; Selvaraj, S; Yue, F; Kim, A; Li, Y; Shen, Y; Hu, M; Liu, J. S.; Ren, B (2012). "Topological domains in mammalian genomes identified by analysis of chromatin interactions". Nature. 485 (7398): 376–80. Bibcode:2012Natur.485..376D. doi:10.1038/nature11082. PMC 3356448. PMID 22495300.
  5. ^ Krijger, Peter Hugo Lodewijk; de Laat, Wouter (2016). "Regulation of disease-associated gene expression in the 3D genome". Nature Reviews. Molecular Cell Biology. 17 (12): 771–782. doi:10.1038/nrm.2016.138. ISSN 1471-0080. PMID 27826147.
  6. ^ Ghavi-Helm, Yad; Jankowski, Aleksander; Meiers, Sascha; Viales, Rebecca R.; Korbel, Jan O.; Furlong, Eileen E. M. (2019). "Highly rearranged chromosomes reveal uncoupling between genome topology and gene expression". Nature Genetics. 51 (8): 1272–1282. doi:10.1038/s41588-019-0462-3. ISSN 1546-1718.
  7. ^ pubmeddev. "The three-dimensional cancer genome. - PubMed - NCBI". www.ncbi.nlm.nih.gov. Retrieved 2019-12-04.
  8. ^ Valton, Anne-Laure; Dekker, Job (2016). "TAD disruption as oncogenic driver". Current Opinion in Genetics & Development. 36: 34–40. doi:10.1016/j.gde.2016.03.008. ISSN 1879-0380. PMC 4880504. PMID 27111891.
  9. ^ Achinger-Kawecka, Joanna; Clark, Susan J. (2017). "Disruption of the 3D cancer genome blueprint". Epigenomics. 9 (1): 47–55. doi:10.2217/epi-2016-0111. ISSN 1750-192X. PMID 27936932.
  10. ^ a b Spielmann, Malte; Lupiáñez, Darío G.; Mundlos, Stefan (2018). "Structural variation in the 3D genome". Nature Reviews. Genetics. 19 (7): 453–467. doi:10.1038/s41576-018-0007-0. ISSN 1471-0064. PMID 29692413.
  11. ^ a b Dixon, Jesse R.; Gorkin, David U.; Ren, Bing (2016). "Chromatin Domains: The Unit of Chromosome Organization". Molecular Cell. 62 (5): 668–680. doi:10.1016/j.molcel.2016.05.018. ISSN 1097-4164. PMC 5371509. PMID 27259200.
  12. ^ de Laat, Wouter; Duboule, Denis (23 October 2013). "Topology of mammalian developmental enhancers and their regulatory landscapes". Nature. 502 (7472): 499–506. Bibcode:2013Natur.502..499D. doi:10.1038/nature12753. PMID 24153303.
  13. ^ a b Szabo, Quentin; Bantignies, Frédéric; Cavalli, Giacomo (10 April 2019). "Principles of genome folding into topologically associating domains". Science Advances. 5 (4): eaaw1668. doi:10.1126/sciadv.aaw1668.
  14. ^ Sexton, Tom; Yaffe, Eitan; Kenigsberg, Ephraim; Bantignies, Frédéric; Leblanc, Benjamin; Hoichman, Michael; Parrinello, Hugues; Tanay, Amos; Cavalli, Giacomo (February 2012). "Three-Dimensional Folding and Functional Organization Principles of the Drosophila Genome". Cell. 148 (3): 458–472. doi:10.1016/j.cell.2012.01.010. PMID 22265598.
  15. ^ Wang, Yanli; Song, Fan; Zhang, Bo; Zhang, Lijun; Xu, Jie; Kuang, Da; Li, Daofeng; Choudhary, Mayank N. K.; Li, Yun; Hu, Ming; Hardison, Ross (2018-10-04). "The 3D Genome Browser: a web-based browser for visualizing 3D genome organization and long-range chromatin interactions". Genome Biology. 19 (1): 151. doi:10.1186/s13059-018-1519-9. ISSN 1474-760X. PMC 6172833. PMID 30286773.{{cite journal}}: CS1 maint: PMC format (link) CS1 maint: unflagged free DOI (link)
  16. ^ Yang, Dongchan; Jang, Insu; Choi, Jinhyuk; Kim, Min-Seo; Lee, Andrew J.; Kim, Hyunwoong; Eom, Junghyun; Kim, Dongsup; Jung, Inkyung; Lee, Byungwook (2018). "3DIV: A 3D-genome Interaction Viewer and database". Nucleic Acids Research. 46 (D1): D52–D57. doi:10.1093/nar/gkx1017. ISSN 1362-4962. PMC 5753379. PMID 29106613.
  17. ^ Szalaj, Przemyslaw; Michalski, Paul J.; Wróblewski, Przemysław; Tang, Zhonghui; Kadlof, Michal; Mazzocco, Giovanni; Ruan, Yijun; Plewczynski, Dariusz (2016). "3D-GNOME: an integrated web service for structural modeling of the 3D genome". Nucleic Acids Research. 44 (W1): W288–293. doi:10.1093/nar/gkw437. ISSN 1362-4962. PMC 4987952. PMID 27185892.
  18. ^ Racko D, Benedetti F, Dorier J, Stasiak A (13 November 2017). "Transcription-induced supercoiling as the driving force of chromatin loop extrusion during formation of TADs in interphase chromosomes". Nucleic Acids Res. 46 (4): 1648–1660. doi:10.1093/nar/gkx1123. PMC 5829651. PMID 29140466. Material was copied from this source, which is available under a Creative Commons Attribution 4.0 International License.
  19. ^ a b Racko D, Benedetti F, Dorier J, Stasiak A (2018). "Are TADs supercoiled?". Nucleic Acids Res. 47 (2): 521–532. doi:10.1093/nar/gky1091. PMC 6344874. PMID 30395328.
  20. ^ Racko D, Benedetti F, oundaroulis D, Stasiak A (2018). "Chromatin Loop Extrusion and Chromatin Unknotting". Polymers. 10 (10): 1126–1137. doi:10.3390/polym10101126. PMC 6403842.{{cite journal}}: CS1 maint: unflagged free DOI (link)
  21. ^ Dekker, Cees; Haering, Christian H.; Kalichava, Ana; Kim, Eugene; Bisht, Shveta; Shaltiel, Indra A.; Ganji, Mahipal (2018-04-06). "Real-time imaging of DNA loop extrusion by condensin". Science. 360 (6384): 102–105. doi:10.1126/science.aar7831. ISSN 0036-8075. PMC 6329450. PMID 29472443.
  22. ^ a b Jost, Daniel; Vaillant, Cédric; Meister, Peter (February 2017). "Coupling 1D modifications and 3D nuclear organization: data, models and function". Current Opinion in Cell Biology. 44: 20–27. doi:10.1016/j.ceb.2016.12.001. PMID 28040646.
  23. ^ Pope, B. D.; Ryba, T; Dileep, V; Yue, F; Wu, W; Denas, O; Vera, D. L.; Wang, Y; Hansen, R. S.; Canfield, T. K.; Thurman, R. E.; Cheng, Y; Gülsoy, G; Dennis, J. H.; Snyder, M. P.; Stamatoyannopoulos, J. A.; Taylor, J; Hardison, R. C.; Kahveci, T; Ren, B; Gilbert, D. M. (2014). "Topologically associating domains are stable units of replication-timing regulation". Nature. 515 (7527): 402–5. Bibcode:2014Natur.515..402P. doi:10.1038/nature13986. PMC 4251741. PMID 25409831.
  24. ^ Ji, X; Dadon, DB; Powell, BE; Fan, ZP; Borges-Rivera, D; Shachar, S; Weintraub, AS; Hnisz, D; Pegoraro, G; Lee, TI; Misteli, T; Jaenisch, R; Young, RA (4 February 2016). "3D Chromosome Regulatory Landscape of Human Pluripotent Cells". Cell Stem Cell. 18 (2): 262–75. doi:10.1016/j.stem.2015.11.007. PMC 4848748. PMID 26686465.
  25. ^ Lupiáñez, Darío G.; Spielmann, Malte; Mundlos, Stefan (April 2016). "Breaking TADs: How Alterations of Chromatin Domains Result in Disease". Trends in Genetics. 32 (4): 225–237. doi:10.1016/j.tig.2016.01.003. hdl:11858/00-001M-0000-002E-1D1D-D. PMID 26862051.
  26. ^ Lupiáñez, D. G.; Kraft, K; Heinrich, V; Krawitz, P; Brancati, F; Klopocki, E; Horn, D; Kayserili, H; Opitz, J. M.; Laxova, R; Santos-Simarro, F; Gilbert-Dussardier, B; Wittler, L; Borschiwer, M; Haas, S. A.; Osterwalder, M; Franke, M; Timmermann, B; Hecht, J; Spielmann, M; Visel, A; Mundlos, S (2015). "Disruptions of Topological Chromatin Domains Cause Pathogenic Rewiring of Gene-Enhancer Interactions". Cell. 161 (5): 1012–1025. doi:10.1016/j.cell.2015.04.004. PMC 4791538. PMID 25959774.
  27. ^ Angier, Natalie (2017-01-09). "A Family's Shared Defect Sheds Light on the Human Genome". The New York Times.
  28. ^ Franke, Martin; Ibrahim, Daniel M.; Andrey, Guillaume; Schwarzer, Wibke; Heinrich, Verena; Schöpflin, Robert; Kraft, Katerina; Kempfer, Rieke; Jerković, Ivana (October 2016). "Formation of new chromatin domains determines pathogenicity of genomic duplications". Nature. 538 (7624): 265–269. Bibcode:2016Natur.538..265F. doi:10.1038/nature19800. ISSN 1476-4687. PMID 27706140.
  29. ^ Hnisz, Denes; Weintraub, Abraham S.; Day, Daniel S.; Valton, Anne-Laure; Bak, Rasmus O.; Li, Charles H.; Goldmann, Johanna; Lajoie, Bryan R.; Fan, Zi Peng (2016-03-03). "Activation of proto-oncogenes by disruption of chromosome neighborhoods". Science. 351 (6280): 1454–1458. Bibcode:2016Sci...351.1454H. doi:10.1126/science.aad9024. ISSN 0036-8075. PMC 4884612. PMID 26940867.
  30. ^ Flavahan, William A.; Drier, Yotam; Liau, Brian B.; Gillespie, Shawn M.; Venteicher, Andrew S.; Stemmer-Rachamimov, Anat O.; Suvà, Mario L.; Bernstein, Bradley E. (2016-01-07). "Insulator dysfunction and oncogene activation in IDH mutant gliomas". Nature. 529 (7584): 110–114. Bibcode:2016Natur.529..110F. doi:10.1038/nature16490. ISSN 0028-0836. PMC 4831574. PMID 26700815.
  31. ^ Weischenfeldt, Joachim; Dubash, Taronish; Drainas, Alexandros P.; Mardin, Balca R.; Chen, Yuanyuan; Stütz, Adrian M.; Waszak, Sebsatian M.; Bosco, Graziella; Halvorsen, Ann R.; Raeder, Benjamin; Efthymiopoulos, Theocharis; Erkek, Serap; Siegl, Christine; Brenner, Hermann; Brustugun, Odd T.; Dieter, Sebastian M; Northcott, Paul A.; Petersen, Iver; Pfister, Stefan M.; Schneider, Martin; Solberg, Steinar K.; Thunissen, Erik; Weichert, Wilko; Zichner, Thomas; Thomas, Roman; Peifer, Martin; Helland, Aslaug; Ball, Claudia R.; Jechlinger, Martin; Sotillo, Rocio; Glimm, Hanno; Korbel, Jan O. (2016). "Pan-cancer analysis of somatic copy-number alterations implicates IRS4 and IGF2 in enhancer hijacking". Nature Genetics. 49 (1): 65–74. doi:10.1038/ng.3722. PMC 5791882. PMID 27869826.
  32. ^ a b Gonzalez-Sandoval, Adriana; Gasser, Susan M. (August 2016). "On TADs and LADs: Spatial Control Over Gene Expression". Trends in Genetics. 32 (8): 485–495. doi:10.1016/j.tig.2016.05.004. ISSN 0168-9525. PMID 27312344.
  33. ^ Li, Mo; Liu, Guang-Hui; Izpisua Belmonte, Juan Carlos (2012-07-23). "Navigating the epigenetic landscape of pluripotent stem cells". Nature Reviews Molecular Cell Biology. 13 (8): 524–535. doi:10.1038/nrm3393. ISSN 1471-0080. PMID 22820889.

outside the TAD.[1] These three-dimensional chromosome structures are present in animals as well as some plants, fungi, and bacteria. In bacteria, they are referred to as Chromosomal Interacting Domains (CIDs).[2] TADs can range in size from thousands to millions of DNA bases.

The functions of TADs are not fully understood, but in some cases, disrupting TADs leads to disease because changing the 3D organization of the chromosome disrupts gene regulation. The mechanisms underlying TAD formation are also complex and not yet fully elucidated, though a number of protein complexes and DNA elements are associated with TAD boundaries.

Discovery and definition[edit]

TADs are defined as regions whose DNA sequences preferentially contact each other. They were discovered in 2012 using chromosome conformation capture techniques including Hi-C.[3][4][5] They have been shown to be present in fruit flies (Drosophila),[6] mouse[3] and human[5] genomes, but not in the wine yeast Saccharomyces cerevisiae.[1]

TAD locations are defined by applying an algorithm to Hi-C data. For example, TADs are often called according to the so-called "directionality index".[5] The directionality index is calculated for individual 40kb bins, by collecting the reads that fall in the bin, and observing whether their paired reads map upstream or downstream of the bin (read pairs are required to span no more than 2Mb). A positive value indicates that more read pairs lie downstream than upstream, and a negative value indicates the reverse. Mathematically, the directionality index is a signed chi-square statistic.

Mechanisms of formation[edit]

DNA loop extrusion through cohesin rings

A number of proteins are known to be associated with TAD formation including the protein CTCF and the protein complex cohesin.[1] It is also unknown what components are required at TAD boundaries; however, in mammalian cells, it has been shown that these boundary regions have comparatively high levels of CTCF binding. In addition, some types of genes (such as transfer RNA genes and housekeeping genes) appear near TAD boundaries more often than would be expected by chance.[3][5]

Computer simulations have shown that chromatin loop extrusion driven by transcription generated supercoiling ensures that cohesin relocalizes quickly and loops grow with reasonable speed and in a good direction. In addition, the supercoiling-driven loop extrusion mechanism is consistent with earlier explanations proposing why TADs flanked by convergent CTCF binding sites form more stable chromatin loops than TADs flanked by divergent CTCF binding sites. In this model, the supercoiling also stimulates enhancer promoter contacts and it is proposed that transcription of eRNA sends the first wave of supercoiling that can activate mRNA transcription in a given TAD.[7][8] Computational models also showed that cohesin rings act like a very efficient molecular comb, pushing knots and entanglements such as in catenanes towards border of TADs where these are removed by the action of topoisomerases. Consistently, removal of entanglements during loop extrusion also increases degree of segregation between chromosomes.[9] However, proof for DNA loop-extrusion is so far limited to condensin (cohesin's sister protein complex) only.[10]

Properties[edit]

Conservation[edit]

TADs have been reported to be relatively constant between different cell types (in stem cells and blood cells, for example), and even between species in specific cases.[11]

Relationship with promoter-enhancer contacts[edit]

The majority of observed interactions between promoters and enhancers do not cross TAD boundaries. Removing a TAD boundary (for example, using CRISPR to delete the relevant region of the genome) can allow new promoter-enhancer contacts to form. This can affect gene expression nearby - such misregulation has been shown to cause limb malformations (e.g. polydactyly) in humans and mice.[11]

Computer simulations have shown that transcription-induced supercoiling of chromatin fibres can explain how TADs are formed and how they can assure very efficient interactions between enhancers and their cognate promoters located in the same TAD.[8]

Relationship with other structural features of the genome[edit]

TADs have been reported to be the same as replication domains, regions of the genome that are copied (replicated) at the same time during S phase of cell division.[12] Insulated neighborhoods, DNA loops formed by CTCF/cohesin-bound regions, are proposed to functionally underlie TADs.[13]

Role in disease[edit]

Disruption of TAD boundaries can affect the expression of nearby genes, and this can cause disease.[14]

For example, genomic structural variants that disrupt TAD boundaries have been reported to cause developmental disorders such as human limb malformations.[15][16][17] Additionally, several studies have provided evidence that the disruption or rearrangement of TAD boundaries can provide growth advantages to certain cancers, such as T-cell acute lymphoblastic leukemia (T-ALL),[18] gliomas,[19] and lung cancer.[20]

Lamina-associated domains[edit]

LADs (dark gray lines) and proteins that interact with them. Lamina is indicated by green curve.
Main article: Nuclear lamina

Lamina-associated domains (LADs) are parts of the chromatin that heavily interact with the lamina, a network-like structure at the inner membrane of the nucleus.[21] LADs consist mostly of transcriptionally silent chromatin, being enriched with trimethylated Lys27 on histone H3, which is a common posttranslational histone modification of heterochromatin.[22] LADs have CTCF-binding sites at their periphery.[21]

See also[edit]

References[edit]

  1. ^ a b c Pombo, A; Dillon, N (April 2015). "Three-dimensional genome architecture: players and mechanisms". Nature Reviews Molecular Cell Biology. 16 (4): 245–57. doi:10.1038/nrm3965. PMID 25757416.
  2. ^ Szabo, Quentin; Bantignies, Frédéric; Cavalli, Giacomo (10 April 2019). "Principles of genome folding into topologically associating domains". Science Advances. 5 (4): eaaw1668. doi:10.1126/sciadv.aaw1668.
  3. ^ a b c Nora, Elphège P.; Lajoie, Bryan R.; Schulz, Edda G.; Giorgetti, Luca; Okamoto, Ikuhiro; Servant, Nicolas; Piolot, Tristan; Van Berkum, Nynke L.; Meisig, Johannes; Sedat, John; Gribnau, Joost; Barillot, Emmanuel; Blüthgen, Nils; Dekker, Job; Heard, Edith (2012). "Spatial partitioning of the regulatory landscape of the X-inactivation centre". Nature. 485 (7398): 381–385. Bibcode:2012Natur.485..381N. doi:10.1038/nature11049. PMC 3555144. PMID 22495304.
  4. ^ de Laat, Wouter; Duboule, Denis (23 October 2013). "Topology of mammalian developmental enhancers and their regulatory landscapes". Nature. 502 (7472): 499–506. Bibcode:2013Natur.502..499D. doi:10.1038/nature12753. PMID 24153303.
  5. ^ a b c d Dixon, J. R.; Selvaraj, S; Yue, F; Kim, A; Li, Y; Shen, Y; Hu, M; Liu, J. S.; Ren, B (2012). "Topological domains in mammalian genomes identified by analysis of chromatin interactions". Nature. 485 (7398): 376–80. Bibcode:2012Natur.485..376D. doi:10.1038/nature11082. PMC 3356448. PMID 22495300.
  6. ^ Sexton, Tom; Yaffe, Eitan; Kenigsberg, Ephraim; Bantignies, Frédéric; Leblanc, Benjamin; Hoichman, Michael; Parrinello, Hugues; Tanay, Amos; Cavalli, Giacomo (February 2012). "Three-Dimensional Folding and Functional Organization Principles of the Drosophila Genome". Cell. 148 (3): 458–472. doi:10.1016/j.cell.2012.01.010. PMID 22265598.
  7. ^ Racko D, Benedetti F, Dorier J, Stasiak A (13 November 2017). "Transcription-induced supercoiling as the driving force of chromatin loop extrusion during formation of TADs in interphase chromosomes". Nucleic Acids Res. 46 (4): 1648–1660. doi:10.1093/nar/gkx1123. PMC 5829651. PMID 29140466. Material was copied from this source, which is available under a Creative Commons Attribution 4.0 International License.
  8. ^ a b Racko D, Benedetti F, Dorier J, Stasiak A (2018). "Are TADs supercoiled?". Nucleic Acids Res. 47 (2): 521–532. doi:10.1093/nar/gky1091. PMC 6344874. PMID 30395328.
  9. ^ Racko D, Benedetti F, oundaroulis D, Stasiak A (2018). "Chromatin Loop Extrusion and Chromatin Unknotting". Polymers. 10 (10): 1126–1137. doi:10.3390/polym10101126. PMC 6403842.{{cite journal}}: CS1 maint: unflagged free DOI (link)
  10. ^ Dekker, Cees; Haering, Christian H.; Kalichava, Ana; Kim, Eugene; Bisht, Shveta; Shaltiel, Indra A.; Ganji, Mahipal (2018-04-06). "Real-time imaging of DNA loop extrusion by condensin". Science. 360 (6384): 102–105. doi:10.1126/science.aar7831. ISSN 0036-8075. PMC 6329450. PMID 29472443.
  11. ^ a b Jost, Daniel; Vaillant, Cédric; Meister, Peter (February 2017). "Coupling 1D modifications and 3D nuclear organization: data, models and function". Current Opinion in Cell Biology. 44: 20–27. doi:10.1016/j.ceb.2016.12.001. PMID 28040646.
  12. ^ Pope, B. D.; Ryba, T; Dileep, V; Yue, F; Wu, W; Denas, O; Vera, D. L.; Wang, Y; Hansen, R. S.; Canfield, T. K.; Thurman, R. E.; Cheng, Y; Gülsoy, G; Dennis, J. H.; Snyder, M. P.; Stamatoyannopoulos, J. A.; Taylor, J; Hardison, R. C.; Kahveci, T; Ren, B; Gilbert, D. M. (2014). "Topologically associating domains are stable units of replication-timing regulation". Nature. 515 (7527): 402–5. Bibcode:2014Natur.515..402P. doi:10.1038/nature13986. PMC 4251741. PMID 25409831.
  13. ^ Ji, X; Dadon, DB; Powell, BE; Fan, ZP; Borges-Rivera, D; Shachar, S; Weintraub, AS; Hnisz, D; Pegoraro, G; Lee, TI; Misteli, T; Jaenisch, R; Young, RA (4 February 2016). "3D Chromosome Regulatory Landscape of Human Pluripotent Cells". Cell Stem Cell. 18 (2): 262–75. doi:10.1016/j.stem.2015.11.007. PMC 4848748. PMID 26686465.
  14. ^ Lupiáñez, Darío G.; Spielmann, Malte; Mundlos, Stefan (April 2016). "Breaking TADs: How Alterations of Chromatin Domains Result in Disease". Trends in Genetics. 32 (4): 225–237. doi:10.1016/j.tig.2016.01.003. hdl:11858/00-001M-0000-002E-1D1D-D. PMID 26862051.
  15. ^ Lupiáñez, D. G.; Kraft, K; Heinrich, V; Krawitz, P; Brancati, F; Klopocki, E; Horn, D; Kayserili, H; Opitz, J. M.; Laxova, R; Santos-Simarro, F; Gilbert-Dussardier, B; Wittler, L; Borschiwer, M; Haas, S. A.; Osterwalder, M; Franke, M; Timmermann, B; Hecht, J; Spielmann, M; Visel, A; Mundlos, S (2015). "Disruptions of Topological Chromatin Domains Cause Pathogenic Rewiring of Gene-Enhancer Interactions". Cell. 161 (5): 1012–1025. doi:10.1016/j.cell.2015.04.004. PMC 4791538. PMID 25959774.
  16. ^ Angier, Natalie (2017-01-09). "A Family's Shared Defect Sheds Light on the Human Genome". The New York Times.
  17. ^ Franke, Martin; Ibrahim, Daniel M.; Andrey, Guillaume; Schwarzer, Wibke; Heinrich, Verena; Schöpflin, Robert; Kraft, Katerina; Kempfer, Rieke; Jerković, Ivana (October 2016). "Formation of new chromatin domains determines pathogenicity of genomic duplications". Nature. 538 (7624): 265–269. Bibcode:2016Natur.538..265F. doi:10.1038/nature19800. ISSN 1476-4687. PMID 27706140.
  18. ^ Hnisz, Denes; Weintraub, Abraham S.; Day, Daniel S.; Valton, Anne-Laure; Bak, Rasmus O.; Li, Charles H.; Goldmann, Johanna; Lajoie, Bryan R.; Fan, Zi Peng (2016-03-03). "Activation of proto-oncogenes by disruption of chromosome neighborhoods". Science. 351 (6280): 1454–1458. Bibcode:2016Sci...351.1454H. doi:10.1126/science.aad9024. ISSN 0036-8075. PMC 4884612. PMID 26940867.
  19. ^ Flavahan, William A.; Drier, Yotam; Liau, Brian B.; Gillespie, Shawn M.; Venteicher, Andrew S.; Stemmer-Rachamimov, Anat O.; Suvà, Mario L.; Bernstein, Bradley E. (2016-01-07). "Insulator dysfunction and oncogene activation in IDH mutant gliomas". Nature. 529 (7584): 110–114. Bibcode:2016Natur.529..110F. doi:10.1038/nature16490. ISSN 0028-0836. PMC 4831574. PMID 26700815.
  20. ^ Weischenfeldt, Joachim; Dubash, Taronish; Drainas, Alexandros P.; Mardin, Balca R.; Chen, Yuanyuan; Stütz, Adrian M.; Waszak, Sebsatian M.; Bosco, Graziella; Halvorsen, Ann R.; Raeder, Benjamin; Efthymiopoulos, Theocharis; Erkek, Serap; Siegl, Christine; Brenner, Hermann; Brustugun, Odd T.; Dieter, Sebastian M; Northcott, Paul A.; Petersen, Iver; Pfister, Stefan M.; Schneider, Martin; Solberg, Steinar K.; Thunissen, Erik; Weichert, Wilko; Zichner, Thomas; Thomas, Roman; Peifer, Martin; Helland, Aslaug; Ball, Claudia R.; Jechlinger, Martin; Sotillo, Rocio; Glimm, Hanno; Korbel, Jan O. (2016). "Pan-cancer analysis of somatic copy-number alterations implicates IRS4 and IGF2 in enhancer hijacking". Nature Genetics. 49 (1): 65–74. doi:10.1038/ng.3722. PMC 5791882. PMID 27869826.
  21. ^ a b Gonzalez-Sandoval, Adriana; Gasser, Susan M. (August 2016). "On TADs and LADs: Spatial Control Over Gene Expression". Trends in Genetics. 32 (8): 485–495. doi:10.1016/j.tig.2016.05.004. ISSN 0168-9525. PMID 27312344.
  22. ^ Li, Mo; Liu, Guang-Hui; Izpisua Belmonte, Juan Carlos (2012-07-23). "Navigating the epigenetic landscape of pluripotent stem cells". Nature Reviews Molecular Cell Biology. 13 (8): 524–535. doi:10.1038/nrm3393. ISSN 1471-0080. PMID 22820889.

Category:Genetics Category:Nuclear organization

Retrieved from "https://en.wikipedia.org/w/index.php?title=User:Khadem.mahdi/Topologically_associating_domain&oldid=931767851"