Positional changes of pericentromeric heterochromatin and nucleoli in postmitotic Purkinje cells during murine cerebellum development

Solovei, Irina; Grandi, Nicole; Knoth, Rolf; Volk, Benedikt; Cremer, Thomas

doi:10.1159/000078202

Cited by 45 publications

(55 citation statements)

References 15 publications

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“…Although it has been previously shown that the localization, number, and size of major satellite regions change during neural development (Billia et al, 1992;Solovei et al, 2004Solovei et al, , 2009, we now show the first evidence that these changes are accompanied by a change in the chromatin state and transcriptional activity of this region. The major satellite regions are traditionally considered to be "silent" regions located within the heterochromatin and marked by repressive histone modifications.…”

Section: Discussionsupporting

confidence: 40%

“…Histone H3 lysine-4 trimethylation becomes localized to chromocenters during neuronal differentiation Because of the previous observation that the number, location and size of major satellite foci change during neuronal development, we asked whether neuronal differentiation is also accompanied by changes in the chromatin state of these regions (Billia et al, 1992;Solovei et al, 2004Solovei et al, , 2009). We used immunostaining to examine histone modifications, a reflection of chromatin state, in major satellite regions during neuronal differentiation.…”

Section: Resultsmentioning

confidence: 99%

“…However, previous evidence suggests a possible role for major satellite regions during neuronal differentiation. DNA-fluorescence in situ hybridization (DNA-FISH) analysis indicated that the number, localization, and size of major satellite foci change during development of post-mitotic Purkinje neurons or rod photoreceptors (Solovei et al, 2004(Solovei et al, , 2009). Furthermore, long-term potentiation-inducing stimuli were shown to decrease the number of major satellite foci in post-mitotic hippocampal neurons (Billia et al, 1992), and transcripts from major satellite regions have been detected in the developing neocortex (Rudert et al, 1995).…”

Section: Introductionmentioning

confidence: 99%

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Transcriptional Activation of Mouse Major Satellite Regions during Neuronal Differentiation

Kishi

Kondo

Gotoh

2012

Cell Struct. Funct.

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ABSTRACT. Recent studies have revealed various biological functions for repetitive sequences, which make up about half of the human genome. One such sequence, major satellites, which are tandem repetitive sequences adjacent to the centromere, have been shown to be a kinetochore component that plays a role in the formation and function of the pericentric heterochromatin necessary for mitosis. However, it is unknown whether these regions also play a role in post-mitotic cells. Here, we show that, during neuronal differentiation, the heterochromatin domains that include major satellite regions become both enriched with the active histone modification lysine-4 trimethylation of histone H3, and more sensitive to nuclease, both of which suggest increased activation of this area. Further supporting this notion, we also found that transcription from major satellite regions is significantly increased during neuronal differentiation both in vitro and in vivo. These results together suggest that the structural and transcriptional state of major satellite regions changes dramatically during neuronal differentiation, implying that this region might play a role in differentiating neurons.

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Section: Discussionsupporting

confidence: 40%

Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Transcriptional Activation of Mouse Major Satellite Regions during Neuronal Differentiation

Kishi

Kondo

Gotoh

2012

Cell Struct. Funct.

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“…genomic loci. Indeed, the composition of the nuclear lamina, the position and architectural changes of the nucleolus, and the sequestration of genomic loci and regulatory proteins into promyelocytic leukemia (PML) bodies, nuclear speckles, histone locus bodies, transcription factories, Cajal bodies, and others have all been linked to gene regulation across a variety of cell types (Solovei et al 2004;Peric-Hupkes et al 2010;Sleeman and Trinkle-Mulcahy 2014).…”

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confidence: 99%

Building up the nucleus: nuclear organization in the establishment of totipotency and pluripotency during mammalian development

Borsos

Torres-Padilla

2016

Genes Dev.

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In mammals, epigenetic reprogramming, the acquisition and loss of totipotency, and the first cell fate decision all occur within a 3-d window after fertilization from the one-cell zygote to the formation of the blastocyst. These processes are poorly understood in molecular detail, yet this is an essential prerequisite to uncover principles of stem cells, chromatin biology, and thus regenerative medicine. A unique feature of preimplantation development is the drastic genome-wide changes occurring to nuclear architecture. From studying somatic and in vitro cultured embryonic stem cells (ESCs) it is becoming increasingly established that the three-dimensional (3D) positions of genomic loci relative to each other and to specific compartments of the nucleus can act on the regulation of gene expression, potentially driving cell fate. However, the functionality, mechanisms, and molecular characteristics of the changes in nuclear organization during preimplantation development are only now beginning to be unraveled. Here, we discuss the peculiarities of nuclear compartments and chromatin organization during mammalian preimplantation development in the context of the transition from totipotency to pluripotency.Totipotency is the capacity to form all cells in a new organism, including embryonic and extraembryonic tissues. A totipotent zygote is created with the fusion of two highly differentiated cells: the oocyte and the sperm that undergoes epigenetic reprogramming. Upon fertilization, the oocyte completes the second meiotic division, and the maternal chromosomes and the sperm chromatin decondense to form separate pronuclei. The paternal chromatin is quickly assembled into nucleosomes upon removal of the sperm-derived protamines. In contrast, the maternal chromatin inherits a nucleosomal configuration from oogenesis. The subsequent cell divisions are termed cleavages because the size of the daughter cells remains approximately half the size of their mother cells (Aiken et al. 2004). After five divisions, the mouse embryo reaches the blastocyst stage, which is initially composed of the inner cell mass (ICM) and the trophectoderm. While the ICM is pluripotent, the trophectoderm is considered a differentiated, epithelia-like tissue. Thus, the transition from a totipotent state in the zygote to a pluripotent state in the blastocyst occurs in only ∼3 d. Although nuclear size progressively shrinks from the zygote to the blastocyst stage, the nucleocytoplasmic ratio increases due to the cleavage nature of divisions. Another peculiarity of preimplantation development is the inheritance of a large protein pool from the oocyte, which enables the earliest steps of development until the embryo undergoes the maternal-to-zygotic transition and activates its own genome.Nuclear organization refers to the spatial position of nuclear compartments as well as the position that specific regions of the genome adopt with respect to each other and the nuclear compartments. Functionally, increasing evidence suggests that the three-dimensional (...

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“…Live-cell observations of movements of a GFP-tagged transgene array in a mammalian cell line (CHO) yielded long-range movements over distances of 1-5 m at velocities from 0.1 to 0.9 m/min (34). Large-scale movements were also observed in nuclei during postmitotic cell differentiation, but these movements required a time scale of days rather than hours (35). In conclusion, it seems unlikely that directed chromatin movements of an extent required for kissing events between widely separated loci take place during interphase.…”

Section: Discussionmentioning

confidence: 84%

Maintenance of imprinting and nuclear architecture in cycling cells

Teller

Solovei

Buiting

et al. 2007

Proc. Natl. Acad. Sci. U.S.A.

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(14) provided a first case-in-point. They performed FISH experiments in normal, phytohemagglutinin (PHA)-stimulated human lymphocytes with a probe covering a segment of the Angelman syndrome/Prader-Willi syndrome (AS/PWS) locus on HSA 15q11-13 and measured 3D interdistances between the two signals in samples of 50 nuclei at different interphase stages. Approximately 38% of nuclei at G 1 , Ϸ18% at early S phase, Ϸ58% at late S phase, and Ϸ18% at G 2 revealed distances Յ2 m, which were considered as a proximity criterion for a possible functional interaction between the two AS/PWS loci. Notably, the significant increase of associations at late S phase was not found in cells from PWS and AS patients. Furthermore, LaSalle and Lalande (14) mentioned that they obtained similar results for the Beckwith-Wiedemann syndrome (BWS) locus, a second imprinted locus on HSA 11p15.5. Based on these findings, LaSalle and Lalande formulated the kissing hypothesis, which states that a transient spatial association between the oppositely imprinted regions during late S phase is a necessary condition to maintain the imprinted status of cycling cells from one cell cycle to the next. This hypothesis was widely cited and further supported by a 2D FISH study from Riesselmann and Haaf (15), who measured 2D interhomolog distances between oppositely imprinted loci on MMU 7 as a fraction of the nuclear diameter in flattened mouse fibroblast nuclei obtained in cytospin preparations. Somatic pairing was assumed when hybridization signals apparently overlapped or touched each other. By this criterion, significantly higher values were found for BrdU-positive nuclei (13%; 27/208 nuclei) compared with BrdUnegative nuclei (9.2%; 21 of 228 nuclei). No increase of pairing frequencies during S phase was found for control regions not subject to imprinting. In contrast, Nogami et al. (16), who studied the frequency of associations between the two AS loci with probes for the imprinted SNRPN alleles in 3D preserved interphase nuclei of human myeloid leukemia HL60 cells, did not find evidence to further support the hypothesis.Importantly, a large variability of 3D positions was noted for pairs of HSA 11 and HSA 15 chromosome territories (CTs) both within nuclei and between nuclei of different cells. Given this variability, a transient kissing event during late S phase between loci widely separated at other stages of interphase requires specific, long-range, directed chromatin movements. The present study was initiated with the intent to clarify whether such movements lead to the transient juxtaposition of entire homologous CTs or, alternatively, whether homologous CTs stay in place, whereas giant loops harboring genes poised for a kissing event expand from territory surfaces and meet each other in between (1,6,8,17). We visualized the two AS/PWS regions in PHA-stimulated lymphocytes by 3D-FISH with a BAC contig covering most of the AS/PWS locus and measured the 3D distances between the two regions in G 1 , early, mid, and late S phase, G 2 , as well as in...

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Positional changes of pericentromeric heterochromatin and nucleoli in postmitotic Purkinje cells during murine cerebellum development

Cited by 45 publications

References 15 publications

Transcriptional Activation of Mouse Major Satellite Regions during Neuronal Differentiation

Transcriptional Activation of Mouse Major Satellite Regions during Neuronal Differentiation

Building up the nucleus: nuclear organization in the establishment of totipotency and pluripotency during mammalian development

Maintenance of imprinting and nuclear architecture in cycling cells

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