Your search keyword '"Koya Odaira"' showing total 5 results

1. <scp>ZNF</scp> 384‐fusion proteins have high affinity for the transcriptional coactivator <scp>EP</scp> 300 and aberrant transcriptional activities

Author

Koya Odaira, Tomoki Naoe, Fumihiko Hayakawa, Takanobu Morishita, Yuki Kojima, Naoyuki Tange, Hitoshi Kiyoi, Yuka Minamikawa, Takahiko Yasuda, Daiki Hirano, Shinobu Tsuzuki, and Hideyuki Yamamoto

Subjects

Adult, Transcriptional Activation, Adolescent, Oncogene Proteins, Fusion, THP-1 Cells, Biophysics, ZNF384, Biochemistry, Fusion gene, 03 medical and health sciences, Structural Biology, SALL4, Genetics, Humans, Promoter Regions, Genetic, EP300, Enhancer, Molecular Biology, Gene, Inhibitor of Differentiation Protein 2, 030304 developmental biology, 0303 health sciences, Chemistry, 030302 biochemistry & molecular biology, Cell Biology, Precursor Cell Lymphoblastic Leukemia-Lymphoma, Fusion protein, Cell biology, Gene Expression Regulation, Neoplastic, Enhancer Elements, Genetic, HEK293 Cells, Transcriptional Coactivator, Trans-Activators, E1A-Associated p300 Protein, Transcription Factors

Abstract

Zinc-finger protein 384 (ZNF384) fusion (Z-fusion) genes have recently been identified as recurrent fusion genes in B-cell precursor acute lymphoblastic leukaemia (BCP-ALL) and have been detected in 7-17% of Philadelphia chromosome-negative BCP-ALL cases. We selected SALL4 and ID2 as potential Z-fusion-specific transcriptional targets that might lead to the differentiation disorder of Z-fusion-positive ALL. The introduction of EP300-ZNF384 and SYNRG-ZNF384 induced the expression of these genes. Z-fusion proteins exhibited stronger transcriptional activities on the promoter or enhancer region of these genes than Wild-Z. Furthermore, GST pull-down assay revealed that Z-fusion proteins associated more strongly with EP300 than Wild-Z. Coexpression of EP300 specifically enhanced the transcriptional activities of Z-fusion proteins. We propose the increased EP300 binding of Z-fusion proteins as a mechanism for their increased transcriptional activities.

Published

2019

2. Periosteum-derived podoplanin-expressing stromal cells regulate nascent vascularization during epiphyseal marrow development

Author

Shogo Tamura, Masato Mukaide, Yumi Katsuragi, Wataru Fujii, Koya Odaira, Nobuaki Suzuki, Nagaharu Tsukiji, Shuichi Okamoto, Atsuo Suzuki, Takeshi Kanematsu, Akira Katsumi, Akira Takagi, Katsuhide Ikeda, Jun Ueyama, Masaaki Hirayama, Katsue Suzuki-Inoue, Tadashi Matsushita, Tetsuhito Kojima, and Fumihiko Hayakawa

Subjects

Membrane Glycoproteins, Bone Marrow, Periosteum, Human Umbilical Vein Endothelial Cells, Endothelial Cells, Humans, Cell Biology, Stromal Cells, Molecular Biology, Biochemistry

Abstract

Bone marrow development and endochondral bone formation occur simultaneously. During endochondral ossification, periosteal vasculatures and stromal progenitors invade the primary avascular cartilaginous anlage, which induces primitive marrow development. We previously determined that bone marrow podoplanin (PDPN)-expressing stromal cells exist in the perivascular microenvironment and promote megakaryopoiesis and erythropoiesis. In this study, we aimed to examine the involvement of PDPN-expressing stromal cells in postnatal bone marrow generation. Using histological analysis, we observed that periosteum-derived PDPN-expressing stromal cells infiltrated the cartilaginous anlage of the postnatal epiphysis and populated on the primitive vasculature of secondary ossification center. Furthermore, immunophenotyping and cellular characteristic analyses indicated that the PDPN-expressing stromal cells constituted a subpopulation of the skeletal stem cell lineage. In vitro xenovascular model cocultured with human umbilical vein endothelial cells and PDPN-expressing skeletal stem cell progenies showed that PDPN-expressing stromal cells maintained vascular integrity via the release of angiogenic factors and vascular basement membrane-related extracellular matrices. We show that in this process, Notch signal activation committed the PDPN-expressing stromal cells into a dominant state with basement membrane-related extracellular matrices, especially type IV collagens. Our findings suggest that the PDPN-expressing stromal cells regulate the integrity of the primitive vasculatures in the epiphyseal nascent marrow. To the best of our knowledge, this is the first study to comprehensively examine how PDPN-expressing stromal cells contribute to marrow development and homeostasis.

Published

2022

3. Staurosporine and venetoclax induce the caspase-dependent proteolysis of MEF2D-fusion proteins and apoptosis in MEF2D-fusion (+) ALL cells

Author

Takahiko Yasuda, Hitoshi Kiyoi, Shinobu Tsuzuki, Naoyuki Tange, Koya Odaira, Seitaro Terakura, Hideyuki Yamamoto, Fumihiko Hayakawa, Daiki Hirano, and Toshiyasu Sakai

Subjects

0301 basic medicine, Proteolysis, Antineoplastic Agents, Apoptosis, RM1-950, Acute lymphoblastic leukemia, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Cell Line, Tumor, High throughput screening, medicine, Staurosporine, Humans, MEF2D, Caspase, Pharmacology, Sulfonamides, medicine.diagnostic_test, biology, Dose-Response Relationship, Drug, Venetoclax, Activator (genetics), MEF2 Transcription Factors, Drug discovery, Drug repositioning, General Medicine, Precursor Cell Lymphoblastic Leukemia-Lymphoma, Bridged Bicyclo Compounds, Heterocyclic, Fusion protein, Molecular biology, 030104 developmental biology, HEK293 Cells, Proteasome, chemistry, 030220 oncology & carcinogenesis, Caspases, biology.protein, Therapeutics. Pharmacology, Gene Fusion, medicine.drug, Signal Transduction

Abstract

MEF2D-fusion (M-fusion) genes are newly discovered recurrent gene abnormalities that are detected in approximately 5 % of acute lymphoblastic leukemia (ALL) cases. Their introduction to cells has been reported to transform cell lines or increase the colony formation of bone marrow cells, suggesting their survival-supporting ability, which prompted us to examine M-fusion-targeting drugs. To identify compounds that reduce the protein expression level of MEF2D, we developed a high-throughput screening system using 293T cells stably expressing a fusion protein of MEF2D and luciferase, in which the protein expression level of MEF2D was easily measured by a luciferase assay. We screened 3766 compounds with known pharmaceutical activities using this system and selected staurosporine as a potential inducer of the proteolysis of MEF2D. Staurosporine induced the proteolysis of M-fusion proteins in M-fusion (+) ALL cell lines. Proteolysis was inhibited by caspase inhibitors, not proteasome inhibitors, suggesting caspase dependency. Consistent with this result, the growth inhibitory effects of staurosporine were stronger in M-fusion (+) ALL cell lines than in negative cell lines, and caspase inhibitors blocked apoptosis induced by staurosporine. We identified the cleavage site of MEF2D-HNRNPUL1 by caspases and confirmed that its caspase cleavage-resistant mutant was resistant to staurosporine-induced proteolysis. Based on these results, we investigated another Food and Drug Administration-approved caspase activator, venetoclax, and found that it exerted similar effects to staurosporine, namely, the proteolysis of M-fusion proteins and strong growth inhibitory effects in M-fusion (+) ALL cell lines. The present study provides novel insights into drug screening strategies and the clinical indications of venetoclax.

Published

2020

4. Aberrant X chromosomal rearrangement through multi‐step template switching during sister chromatid formation in a patient with severe hemophilia A

Author

Tetsuhito Kojima, Akira Takagi, Shuichi Okamoto, Nobuaki Suzuki, Akira Katsumi, Koya Odaira, Takeshi Kanematsu, Mahiru Tokoro, Sachiko Suzuki, Atsuo Suzuki, Shogo Tamura, Tadashi Matsushita, Yuna Hattori, Misaki Kakihara, and Fumihiko Hayakawa

Subjects

Male, 0301 basic medicine, chromosomal rearrangement, lcsh:QH426-470, homologous recombination, Chromosomal rearrangement, Chromatids, 030105 genetics & heredity, Biology, Hemophilia A, Chromosome Breakpoints, inversion, 03 medical and health sciences, Genetics, Homologous chromosome, Humans, Sister chromatids, Molecular Biology, Genetics (clinical), X chromosome, Chromosomes, Human, X, Factor XIII, Breakpoint, Intron, Infant, Original Articles, Introns, Telomere, lcsh:Genetics, 030104 developmental biology, Chromosome Inversion, Original Article, FoSTeS/MMBIR, Homologous recombination, F8

Abstract

Background Hemophilia A (HA) is an X‐linked recessive bleeding disorder caused by pathogenic variants of the coagulation factor VIII gene (F8). Half of the patients with severe HA have a recurrent inversion in the X chromosome, that is, F8 intron 22 or intron 1 inversion. Here, we characterized an abnormal F8 due to atypical complex X chromosome rearrangements in a Japanese patient with severe HA. Methods Recurrent F8 inversions were tested with inverse shifting‐PCR. The genomic structure was investigated using PCR‐based direct sequencing or quantitative PCR. Results The proband's X chromosome had a 119.5 kb insertion, a reverse duplex of an extragenic sequence on the F8 telomere region into the F8 intron 1 with two breakpoints. The telomeric breakpoint was a joining from the F8 intron 1 to the inverted FUNDC2 via a two‐base microhomology, and the centromeric breakpoint was a recombination between F8 intron 1 homologous sequences. The rearrangement mechanism was suggested as a multi‐step rearrangement with template switching such as fork stalling and template switching (FoSTeS)/microhomology‐mediated break‐induced replication (MMBIR) and/or homologous sequence‐associated recombination during a sister chromatid formation. Conclusion We identified the aberrant X chromosome with a split F8 due to a multi‐step rearrangement in a patient with severe HA., Hemophilia A (HA) is an X‐linked recessive bleeding disorder caused by mutations in the coagulation factor VIII gene (F8). We identified the aberrant chromosome X with a split F8 due to a multi‐step rearrangement in a severe HA patient. The rearrangement mechanism was suggested as a multi‐step rearrangement with template switching such as FoSTeS/MMBIR and/or homologous sequence associating recombination during a sister chromatid formation.

Published

2020

5. Apparent synonymous mutation F9 c.87AG causes secretion failure by in-frame mutation with aberrant splicing

Author

Akira Katsumi, Shuichi Okamoto, Mahiru Tokoro, Nobuaki Suzuki, Tetsuhito Kojima, Atsuo Suzuki, Takeshi Kanematsu, Koya Odaira, Akira Takagi, Shogo Tamura, Yuna Hattori, Tadashi Matsushita, Misaki Kakihara, Fumihiko Hayakawa, and Sachiko Suzuki

Subjects

Signal peptide, Silent mutation, Male, Messenger RNA, Expression vector, Chemistry, Mutant, Hematology, 030204 cardiovascular system & hematology, Middle Aged, Molecular biology, Hemophilia B, Factor IX, 03 medical and health sciences, Alternative Splicing, 0302 clinical medicine, 030220 oncology & carcinogenesis, RNA splicing, Mutation, Humans, RNA, Messenger, Synonymous substitution, Gene

Abstract

Introduction Hemophilia B is an X-linked recessive bleeding disorder caused by coagulation factor IX (FIX) gene (F9) mutations. Several F9 synonymous mutations have been known to cause hemophilia B; however, the deleterious mechanisms underlying the development of hemophilia B have not been completely understood. To elucidate the molecular pathogenesis causing hemophilia B, we investigated the synonymous F9 mutation: c.87A>G, p.(Thr29=). Materials and methods The influence of F9 c.87A>G on mRNA splicing was analyzed by exon-trap assay and in silico prediction. We prepared FIX expression vectors using mutant F9 cDNA and transfected HepG2 cells to investigate intracellular transport and extracellular secretion of FIX. Intracellular kinetics of the expressed FIX was examined by treatment with the proteasome inhibitor MG132. Results Exon-trap analysis revealed that F9 c.87A>G resulted in almost (99.1%) aberrant splicing (r.83_88del). In silico analysis predicted that F9 c.87A>G influenced the splicing pattern by generating an available aberrant 5′ splice site. The aberrant F9 mRNA (r.83_88del) was translated to a mutant FIX p.Cys28_Val30delinsPhe with an in-frame mutation at the signal peptide cleavage site. Simultaneously, a small amount (0.9%) of mutant F9 r.87A>G translating into WT FIX p.Thr29 = was also observed. The mutant FIX was abnormally retained in the endoplasmic reticulum (ER) and was not extracellularly secreted. It appeared to be intracellularly degraded via proteasome-dependent degradation machinery. Conclusion F9 c.87A>G was found to cause abnormal mRNA splicing, r.83_88del, and produce the mutant FIX p.Cys28_Val30delinsPhe. The mutant FIX is an abnormal protein with extracellular secretory defects and is intracellularly eliminated via proteasome-dependent ER-associated degradation.

Published

2019