Literature DB >> 8034736

Dynamic changes in the higher-level chromatin organization of specific sequences revealed by in situ hybridization to nuclear halos.

M G Gerdes1, K C Carter, P T Moen, J B Lawrence.   

Abstract

A novel approach to study the higher level packaging of specific DNA sequences has been developed by coupling high-resolution fluorescence hybridization with biochemical fractionation to remove histones and distend DNA loops to form morphologically reproducible nuclear "halos." Results demonstrate consistent differences in the organization of specific sequences, and further suggest a relationship to functional activity. Pulse-incorporated bromodeoxyuridine representing nascent replicating DNA localized with the base of the chromatin loops in discrete clustered patterns characteristic of intact cells, whereas at increasing chase times, the replicated DNA was consistently found further out on the extended region of the halo. Fluorescence hybridization to unique loci for four transcriptionally inactive sequences produced long strings of signal extending out onto the DNA halo or "loop," whereas four transcriptionally active sequences remained tightly condensed as single spots within the residual nucleus. In contrast, in non-extracted cells, all sequences studied typically remained condensed as single spots of fluorescence signal. Interestingly, two transcriptionally active, tandemly repeated gene clusters exhibited strikingly different packaging by this assay. Analysis of specific genes in single cells during the cell cycle revealed changes in packaging between S-phase and non S-phase cells, and further suggested a dramatic difference in the structural associations in mitotic and interphase chromatin. These results are consistent with and suggestive of a loop domain organization of chromatin packaging involving both stable and transient structural associations, and provide precedent for an approach whereby different biochemical fractionation methods may be used to unravel various aspects of the complex higher-level organization of the genome.

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Year:  1994        PMID: 8034736      PMCID: PMC2200020          DOI: 10.1083/jcb.126.2.289

Source DB:  PubMed          Journal:  J Cell Biol        ISSN: 0021-9525            Impact factor:   10.539


  69 in total

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Authors:  J B Lawrence; K C Carter; M J Gerdes
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2.  High-resolution in situ hybridization using DNA halo preparations.

Authors:  J Wiegant; W Kalle; L Mullenders; S Brookes; J M Hoovers; J G Dauwerse; G J van Ommen; A K Raap
Journal:  Hum Mol Genet       Date:  1992-11       Impact factor: 6.150

3.  Genomic organization of human 5 S rDNA and sequence of one tandem repeat.

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5.  A domain model for eukaryotic DNA organization: a molecular basis for cell differentiation and chromosome evolution.

Authors:  J W Bodnar
Journal:  J Theor Biol       Date:  1988-06-22       Impact factor: 2.691

6.  Mapping replicational sites in the eucaryotic cell nucleus.

Authors:  H Nakayasu; R Berezney
Journal:  J Cell Biol       Date:  1989-01       Impact factor: 10.539

7.  A three-dimensional view of precursor messenger RNA metabolism within the mammalian nucleus.

Authors:  K C Carter; D Bowman; W Carrington; K Fogarty; J A McNeil; F S Fay; J B Lawrence
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8.  Fluorescent in situ hybridization of the telomere repeat sequence in hamster sperm nuclear structures.

Authors:  J de Lara; K L Wydner; K M Hyland; W S Ward
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Review 9.  The nuclear matrix: structure and composition.

Authors:  R Verheijen; W van Venrooij; F Ramaekers
Journal:  J Cell Sci       Date:  1988-05       Impact factor: 5.285

10.  Transcriptionally active minichromosomes are attached transiently in nuclei through transcription units.

Authors:  D A Jackson; P R Cook
Journal:  J Cell Sci       Date:  1993-08       Impact factor: 5.285

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  42 in total

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Authors:  H B Sun; J Shen; H Yokota
Journal:  Biophys J       Date:  2000-07       Impact factor: 4.033

2.  Dynamics of association of origins of DNA replication with the nuclear matrix during the cell cycle.

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Journal:  Nucleic Acids Res       Date:  2001-08-01       Impact factor: 16.971

Review 3.  Use of matrix attachment regions (MARs) to minimize transgene silencing.

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5.  Visualization of individual DNA loops and a map of loop domains in the human dystrophin gene.

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Journal:  Nucleic Acids Res       Date:  2004-04-15       Impact factor: 16.971

Review 6.  Heterochromatin instability in cancer: from the Barr body to satellites and the nuclear periphery.

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7.  Performance of genomic bordering elements at predefined genomic loci.

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Journal:  Mol Cell Biol       Date:  2005-03       Impact factor: 4.272

8.  Replication timing of large Sorex granarius (Soricidae, Eulipotyphla) telomeres.

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9.  Loop formation by the transgene WAP:6xHishGH in transgenic rabbit fibroblasts, revealed by fluorescence in situ hybridization to nuclear halos.

Authors:  Ewa Michalak; Daniel Lipiński; Ryszard Słomski
Journal:  J Appl Genet       Date:  2006       Impact factor: 3.240

10.  Identifying Nuclear Matrix-Attached DNA Across the Genome.

Authors:  Jason R Dobson; Deli Hong; A Rasim Barutcu; Hai Wu; Anthony N Imbalzano; Jane B Lian; Janet L Stein; Andre J van Wijnen; Jeffrey A Nickerson; Gary S Stein
Journal:  J Cell Physiol       Date:  2017-01-05       Impact factor: 6.384

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