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Your search keyword '"Tomotoshi Marumoto"' showing total 5 results
Start Over Author "Tomotoshi Marumoto" Publisher springer science and business media llc
5 results on '"Tomotoshi Marumoto"'

1. Development of a novel mouse glioma model using lentiviral vectors

Author

Dinorah Friedmann-Morvinski, Miriam Scadeng, Tomotoshi Marumoto, Fred H. Gage, Yasushi Soda, Ayumu Tashiro, and Inder M. Verma

Subjects
Cell type, Genetic Vectors, Cell, Brain tumor, Hippocampus, Subventricular zone, Mice, SCID, Biology, Models, Biological, Article, General Biochemistry, Genetics and Molecular Biology, Mice, Mice, Inbred NOD, Glioma, medicine, Animals, Humans, Cloning, Molecular, Protein kinase B, Cells, Cultured, Mice, Knockout, Lentivirus, General Medicine, Genes, p53, medicine.disease, Virology, Mice, Inbred C57BL, Transplantation, Disease Models, Animal, medicine.anatomical_structure, Cancer research, HeLa Cells
Abstract

We report the development of a new method to induce glioblastoma multiforme in adult immunocompetent mice by injecting Cre-loxP-controlled lentiviral vectors expressing oncogenes. Cell type- or region-specific expression of activated forms of the oncoproteins Harvey-Ras and AKT in fewer than 60 glial fibrillary acidic protein-positive cells in the hippocampus, subventricular zone or cortex of mice heterozygous for the gene encoding the tumor suppressor Tp53 were tested. Mice developed glioblastoma multiforme when transduced either in the subventricular zone or the hippocampus. However, tumors were rarely detected when the mice were transduced in the cortex. Transplantation of brain tumor cells into naive recipient mouse brain resulted in the formation of glioblastoma multiforme-like tumors, which contained CD133(+) cells, formed tumorspheres and could differentiate into neurons and astrocytes. We suggest that the use of Cre-loxP-controlled lentiviral vectors is a novel way to generate a mouse glioblastoma multiforme model in a region- and cell type-specific manner in adult mice.

Published
2009

2. The tumor suppressor WARTS activates the Omi / HtrA2-dependent pathway of cell death

Author

Tomotoshi Marumoto, Toshihiro Hara, Shin Yonehara, Shinobu Honda, Yoshimi Arima, Naoko Kunitoku, Masanobu Nomura, Shin Ichi Iida, Shinji Kuninaka, Toru Hirota, Hideyuki Saya, Takashi Sasayama, and Kageharu Koja

Subjects
High-Temperature Requirement A Serine Peptidase 2, Cancer Research, Programmed cell death, Tumor suppressor gene, PDZ domain, Apoptosis, Protein Serine-Threonine Kinases, Transfection, medicine.disease_cause, Mitochondrial Proteins, Cytosol, Genetics, medicine, Humans, Molecular Biology, Mitosis, Cells, Cultured, Caspase, biology, Kinase, Tumor Suppressor Proteins, Serine Endopeptidases, fungi, virus diseases, Virology, Mitochondria, Cancer research, biology.protein, Carcinogenesis
Abstract

Drosophila tumor suppressor WARTS (Wts) is an evolutionally conserved serine / threonine kinase and participates in a signaling complex that regulates both proliferation and apoptosis to ensure the proper size and shape of the fly. Human counterparts of this complex have been found to be frequently downregulated or mutated in cancers. WARTS, a human homolog of Wts, is also known as tumor suppressor and mitotic regulator, but its molecular implications in tumorigenesis are still obscure. Here, we show that WARTS binds via its C-terminus to the PDZ domain of a proapoptotic serine protease Omi / HtrA2. Depletion of WARTS inhibited Omi / HtrA2-mediated cell death, whereas overexpression of WARTS promoted this process. Furthermore, WARTS can enhance the protease activity of Omi / HtrA2 both in vivo and in vitro. Activation of Omi / HtrA2-mediated cell death is thus a potential mechanism for the tumor suppressive activity of WARTS.

Published
2005

3. Spindle checkpoint function is required for mitotic catastrophe induced by DNA-damaging agents

Author

Shinobu Honda, Tomotoshi Marumoto, Shinji Kuninaka, Yukitaka Ushio, Masayuki Nitta, Hideyuki Saya, Toru Hirota, and Osamu Kobayashi

Subjects
Cancer Research, Cell cycle checkpoint, Mad2, Base Sequence, Fluorescent Antibody Technique, Mitosis, Biology, G2-M DNA damage checkpoint, Cell biology, Spindle checkpoint, Mitotic exit, Genetics, Humans, Tumor Suppressor Protein p53, Anaphase-promoting complex, Molecular Biology, Mitotic catastrophe, Metaphase, DNA Damage, DNA Primers, HeLa Cells
Abstract

Mitotic catastrophe is an important mechanism for the induction of cell death in cancer cells by antineoplastic agents that damage DNA. This process is facilitated by defects in the G1 and G2 checkpoints of the cell cycle that are apparent in most cancer cells and which allow the cells to enter mitosis with DNA damage. We have now characterized the dynamics of mitotic catastrophe induced by DNA-damaging agents in p53-deficient cancer cells. Cells that entered mitosis with DNA damage transiently arrested at metaphase for more than 10 h without segregation of chromosomes and subsequently died directly from metaphase. In those metaphase arrested precatastrophic cells, anaphase-promoting complex appeared to be inactivated and BubR1 was persistently localized at kinetochores, suggesting that spindle checkpoint is activated after the DNA damage. Furthermore, suppression of spindle checkpoint function by BubR1 or Mad2 RNA interference in the DNA damaged cells led to escape from catastrophic death and to subsequent abnormal mitosis. Dysfunction of the spindle checkpoint in p53-deficient cancer cells is thus likely a critical factor in resistance to DNA-damaging therapeutic agents.

Published
2004

4. Tumor suppressor WARTS ensures genomic integrity by regulating both mitotic progression and G1 tetraploidy checkpoint function

Author

David C. Pallas, Shinji Kuninaka, Toshihiro Hara, Ken-ichiro Kosai, Tomotoshi Marumoto, Shinobu Honda, Toru Hirota, Shin Ichi Iida, Tetsuro Morisaki, Michio Kawasuji, and Hideyuki Saya

Subjects
Cancer Research, Time Factors, Cell cycle checkpoint, Mitosis, Spindle Apparatus, Protein Serine-Threonine Kinases, Biology, Transfection, S Phase, Polyploidy, Genetics, Animals, Drosophila Proteins, Humans, Prometaphase, Molecular Biology, Genome, Ploidies, Cell Cycle, G1 Phase, virus diseases, DNA, Fibroblasts, G2-M DNA damage checkpoint, Cell cycle, Flow Cytometry, Actins, Rats, Spindle apparatus, Cell biology, Spindle checkpoint, Microscopy, Fluorescence, Mitotic exit, Drosophila, Tumor Suppressor Protein p53, Protein Kinases, HeLa Cells
Abstract

Defects in chromosomes or mitotic spindles activate the spindle checkpoint, resulting in cell cycle arrest at prometaphase. The prolonged activation of spindle checkpoint generally leads to mitotic exit without segregation after a transient mitotic arrest and the consequent formation of tetraploid G(1) cells. These tetraploid cells are usually blocked to enter the subsequent S phase by the activation of p53/pRb pathway, which is referred to as the G(1) tetraploidy checkpoint. A human homologue of the Drosophila warts tumor suppressor, WARTS, is an evolutionarily conserved serine-threonine kinase and implicated in development of human tumors. We previously showed that WARTS plays a crucial role in controlling mitotic progression by forming a regulatory complex with zyxin, a regulator of actin filament assembly, on mitotic apparatus. However, when WARTS is activated during cell cycle and how the loss of WARTS function leads to tumorigenesis have not been elucidated. Here we show that WARTS is activated during mitosis in mammalian cells, and that overexpression of a kinase-inactive WARTS in Rat1 fibroblasts significantly induced mitotic delay. This delay resulted from prolonged activation of the spindle assembly checkpoint and was frequently followed by mitotic slippage and the development of tetraploidy. The resulting tetraploid cells then abrogated the G(1) tetraploidy checkpoint and entered S phase to achieve a DNA content of 8N. This impairment of G(1) tetraploidy checkpoint was caused as a consequence of failure to induce p53 expression by expressing a kinase-inactive WARTS. WARTS thus plays a critical role in maintenance of ploidy through its actions in both mitotic progression and the G(1) tetraploidy checkpoint.

Published
2004

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