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Dive into the research topics where Sugako Ogushi is active.

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Featured researches published by Sugako Ogushi.


Science | 2012

Offspring from Oocytes Derived from in Vitro Primordial Germ Cell–like Cells in Mice

Katsuhiko Hayashi; Sugako Ogushi; Kazuki Kurimoto; So Shimamoto; Hiroshi Ohta; Mitinori Saitou

Artificially Induced Oocytes In mice, male embryonic stem cells (ESCs) and induced pluripotent stem cells (iPSCs) have been shown to differentiate into primordial germ cell–like cells (PGCLCs) in vitro. Upon transplantation into testes, these PGCLCs can form fully functional sperm. Again working in mice, Hayashi et al. (p. 971, published online 4 October) found that female ESCs and iPSCs can also differentiate into PGCLCs, which, when aggregated in reconstituted ovaries, exhibited epigenetic reprogramming and meiotic potential in vitro. Upon transplantation of the reconstituted ovaries under ovarian bursa, female PGCLCs developed into fully grown oocytes that contributed to healthy offspring upon in vitro maturation and fertilization. Mature, fully functional female gametes can be generated from mouse pluripotent stem cells. Reconstitution of female germ cell development in vitro is a key challenge in reproductive biology and medicine. We show here that female (XX) embryonic stem cells and induced pluripotent stem cells in mice are induced into primordial germ cell–like cells (PGCLCs), which, when aggregated with female gonadal somatic cells as reconstituted ovaries, undergo X-reactivation, imprint erasure, and cyst formation, and exhibit meiotic potential. Upon transplantation under mouse ovarian bursa, PGCLCs in the reconstituted ovaries mature into germinal vesicle-stage oocytes, which then contribute to fertile offspring after in vitro maturation and fertilization. Our culture system serves as a robust foundation for the investigation of key properties of female germ cells, including the acquisition of totipotency, and for the reconstitution of whole female germ cell development in vitro.


Cell Cycle | 2006

Loss of Rec8 from chromosome arm and centromere region is required for homologous chromosome separation and sister chromatid separation, respectively, in mammalian meiosis.

Jibak Lee; Konosuke Okada; Sugako Ogushi; Takashi Miyano; Masashi Miyake; Masakane Yamashita

Chromosome separation in meiosis I is different from those in mitosis and meiosis II inthat homologs separate from each other in the former while sisters do so in the latter. Weshow here that meiosis-specific cohesin subunit Rec8 in mouse oocytes showsessentially the same pattern of localization to those reported in yeasts1-3 and mammalianspermatocytes4,5; Rec8 along chromosome arm (armRec8) is lost at the metaphaseI-to-anaphase I transition, although centromeric Rec8 (cenRec8) is maintained until theonset of anaphase II. Suppression of the loss of armRec8 by microinjection of anti-Rec8antibody into the oocytes inhibits homolog separation but not the first polar bodyemission (cytokinesis). Similarly, the injection of anti-Rec8 antibody into metaphase IIoocytes prevents sister separation in anaphase II after oocyte activation. These datademonstrate that the loss of armRec8 and cenRec8 is required for separation ofhomologs and sisters, respectively, but both are not required for other late mitotic eventssuch as spindle elongation and cytokinesis in mouse oocytes. Further, we propose thatloss of armRec8 (homolog separation) and cytokinesis are suppressed until anaphase Iby Securin whose destruction is regulated by spindle checkpoint-proteasome pathway,and that Topoisomerase II is required for homolog separation independently from suchpathway.


Molecular Biology of the Cell | 2011

Condensins I and II are essential for construction of bivalent chromosomes in mouse oocytes

Jibak Lee; Sugako Ogushi; Mitinori Saitou; Tatsuya Hirano

In mouse oocytes, condensin I localizes around centromeric regions, whereas condensin II is concentrated onto chromatid axes of Meta-I bivalent chromosomes. Both condensins are required for many aspects of meiotic chromosome dynamics, including individualization, resolution, and segregation, as well as monopolar attachment of sister kinetochores.


Biology of Reproduction | 2011

Involvement of Mouse Nucleoplasmin 2 in the Decondensation of Sperm Chromatin after Fertilization

Azusa Inoue; Sugako Ogushi; Mitinori Saitou; Masataka G. Suzuki; Fugaku Aoki

The tightly condensed chromatin of spermatozoa is rapidly decondensed after the spermatozoa enter oocytes. Although no factor involved in sperm chromatin decondensation (SCD) has been identified in mammals, it has been suggested that a factor related to SCD activity is present in the germinal vesicle (GV) of oocytes. Here, we found that the nucleolus-like body (NLB), which is a component of the GV, is involved in SCD in murine oocytes. When NLBs were microsurgically removed from GV-stage oocytes, SCD was significantly retarded in the paternal genome after fertilization following meiotic maturation. We found that the retardation of SCD in the NLB-removed oocytes was restored by the microinjection of mRNA encoding nucleoplasmin 2 (NPM2), a component of NLBs. Furthermore, SCD was retarded in the fertilized oocytes from Npm2-knockout females, and recombinant NPM2 alone could induce the SCD in vitro. These data provide evidence that NPM2 is involved in sperm chromatin remodeling in mammals.


Molecular Reproduction and Development | 2011

Nucleoli From Growing Oocytes Inhibit the Maturation of Enucleolated, Full-Grown Oocytes in the Pig

Hirohisa Kyogoku; Sugako Ogushi; Takashi Miyano; Josef Fulka

In mammals, the nucleolus of full‐grown oocyte is essential for embryonic development but not for oocyte maturation. In our study, the role of the growing oocyte nucleolus in oocyte maturation was examined by nucleolus removal and/or transfer into previously enucleolated, growing (around 100 µm in diameter) or full‐grown (120 µm) pig oocytes. In the first experiment, the nucleoli were aspirated from growing oocytes whose nucleoli had been compacted by actinomycin D treatment, and the enucleolated oocytes were matured in vitro. Most of non‐treated or actinomycin D‐treated oocytes did not undergo germinal vesicle breakdown (GVBD; 13% and 12%, respectively). However, the GVBD rate of enucleolated, growing oocytes significantly increased to 46%. The low GVBD rate of enucleolated, growing oocytes was restored again by the re‐injection of nucleoli from growing oocytes (23%), but not when nucleoli from full‐grown oocytes were re‐injected into enucleolated, growing oocytes (49%). When enucleolated, full‐grown oocytes were injected with nucleoli from growing or full‐grown oocytes, the nucleolus in the germinal vesicle was reassembled (73% and 60%, respectively). After maturation, the enucleolated, full‐grown oocytes injected with nucleoli from full‐grown oocytes matured to metaphase II (56%), whereas injection with growing‐oocyte nucleoli reduced this maturation to 21%. These results suggest that the growing‐oocyte nucleolus is involved in the oocytes meiotic arrest, and that the full‐grown oocyte nucleolus has lost the ability. Mol. Reprod. Dev. 78:426–435, 2011.


Molecular Reproduction and Development | 2009

Nucleoli from growing oocytes support the development of enucleolated full‐grown oocytes in the pig

Hirohisa Kyogoku; Sugako Ogushi; Takashi Miyano

Recent research has shown that the maternal nucleolus is essential for embryonic development. The morphology of the nucleolus in growing oocytes differs from that in full‐grown oocytes. We determined the ability of nucleoli from growing oocytes to substitute for nucleoli of full‐grown oocytes in terms of supporting embryonic development in this study. Growing (around 100 µm in diameter) and full‐grown porcine oocytes (120 µm) were collected from small (0.6–1.0 mm) and large antral follicles (4–5 mm), respectively. The nucleolus was aspirated from full‐grown oocytes by micromanipulation, and the resulting enucleolated oocytes were matured to metaphase II; the nucleoli originating from full‐grown and growing oocytes were then injected into the oocytes. The Chromatin of growing oocytes was aspirated with the nucleolus during the enucleolation process. Growing oocytes were thus treated with actinomycin D to release the chromatin from their nucleoli, and the nucleoli were collected and transferred to the enucleolated and matured full‐grown oocytes. After activation by electro‐stimulation, nucleoli were formed in pronuclei of sham‐operated oocytes. Enucleolated oocytes that had been injected with nucleoli from either full‐grown or growing, however, did not form any nucleoli in the pronuclei. No enucleolated oocytes developed to blastocysts, whereas enucleolated oocytes injected with nucleoli from full‐grown oocytes (15%) or growing oocytes (18%) developed to blastocysts. These results indicate that the nucleoli from growing oocytes can substitute for nucleoli from full‐grown oocytes during early embryonic development. Mol. Reprod. Dev. 77: 167–173, 2010.


Biology of Reproduction | 2012

Nucleoli from Two-Cell Embryos Support the Development of Enucleolated Germinal Vesicle Oocytes in the Pig

Hirohisa Kyogoku; Sugako Ogushi; Takashi Miyano

ABSTRACT Recent research has shown that nucleoli of oocytes at the germinal vesicle (GV) stage (GV nucleoli) are not necessary for oocyte maturation but are essential for early embryonic development. Nucleoli of 2-cell embryos (2-cell nucleoli) have morphology similar to that of nucleoli in oocytes at the GV stage. In this study, we examined the ability of 2-cell nucleoli to substitute for GV nucleoli in terms of supporting early embryonic development by nucleolus aspiration (enucleolation) and transfer into metaphase II (MII) oocytes or 2-cell embryos that were derived from enucleolated oocytes at the GV stage in the pig. When 2-cell embryos were centrifuged to move the lipid droplets to one side of the blastomere, multiple nucleoli in the nucleus fused into a single nucleolus. The nucleoli were then aspirated from the 2-cell embryos by micromanipulation. The injection of 2-cell nucleoli to GV enucleolated oocytes at the MII stage rescued the embryos from the early embryonic arrest, and the resulting oocytes developed to blastocysts. However, the injection of 2-cell and GV nucleoli to 2-cell embryos derived from GV enucleolated oocytes rarely restored the development to blastocysts. These results indicate that 2-cell nucleoli support early embryonic development as GV nucleoli and that the presence of nucleoli is essential for pig embryos before the 2-cell stage.


Journal of Reproduction and Development | 2010

The Nucleolus in the Mouse Oocyte is Required for the Early Step of Both Female and Male Pronucleus Organization

Sugako Ogushi; Mitinori Saitou


Journal of Reproduction and Development | 2012

Effects of proteasome inhibitors on the nucleolar size of porcine oocytes.

Mayumi Jitsukawa; Hirohisa Kyogoku; Sugako Ogushi; Takashi Miyano


Journal of Reproduction and Development | 2013

Development of Enucleolated Pig Oocytes after Injection of Nucleoli from 2-cell Embryos

Hirohisa Kyogoku; Sugako Ogushi; Takashi Miyano

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Josef Fulka

Czechoslovak Academy of Sciences

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