2026/03/07 更新

写真a

イヌイ マサフミ
乾 雅史
INUI MASAFUMI
所属
学部 農学部 専任教授
職名
専任教授
外部リンク

学位

  • 理学 ( 2006年3月   東京大学 )

研究キーワード

  • ゲノム編集

  • 軟骨

  • 発生生物学

  • 形態形成

  • シグナル伝達

  • 翻訳後修飾

  • 骨格筋

研究分野

  • ライフサイエンス / 発生生物学

  • ライフサイエンス / 分子生物学

学歴

  • Graduate school of Science, The University of Tokyo   Department of Biological Science

    2001年4月 - 2006年3月

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経歴

  • 明治大学   農学部 生命科学科   教授

    2025年4月 - 現在

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  • 明治大学   農学部 生命科学科   准教授

    2020年4月 - 2025年3月

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  • 明治大学   農学部 生命科学科   専任講師

    2017年4月 - 2020年3月

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  • 国立成育医療研究センター   システム発生・再生医学研究部   ゲノム機能研究室長

    2012年 - 2017年3月

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  • Department of Medical Biotechnologies, University of Padua   Section of Histology and Embryology   Post-doctoral fellow

    2006年 - 2012年

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  • Graduate School of Science, The University of Tokyo   Department of Biological Sciences   Ph.D course

    2001年 - 2006年

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▼全件表示

論文

  • SMAD2 ubiquitination through PY motif regulates skeletal muscle mass and fibrotic degeneration 査読

    Yuki Yamasaki, Keita Sakamoto, Shunki Yashiro, Yutaro Kawa, Akiko Kondow, Atsushi Kubo, Keisuke Hitachi, Masafumi Inui

    Scientific Reports   16 ( 1 )   6666   2026年1月

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    担当区分:最終著者, 責任著者   掲載種別:研究論文(学術雑誌)   出版者・発行元:Springer Science and Business Media LLC  

    DOI: 10.1038/s41598-026-37582-z

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    その他リンク: https://www.nature.com/articles/s41598-026-37582-z.pdf

  • Methods for Collecting and Analyzing Post-Ejaculatory Uterine Fluid and the Uterus in Mice. 査読 国際誌

    Yu Matsumoto, Ban Sato, Masafumi Inui, Manato Sunamoto, Natsuko Kawano, Kenji Miyado

    Bio-protocol   15 ( 24 )   e5544   2025年12月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    In mammals, the semen is ejaculated into the female reproductive tract, and the sperm travel to the oviduct to fertilize the egg. A comprehensive understanding of the pre- and post-ejaculatory intrauterine environment is one of the key points for overcoming infertility; however, the dynamics of the intrauterine environment and its physiological role in the uterus, namely in the internal fertilization process, remain unclear. Conventional methods for collecting uterine fluids from the uterus post-ejaculation of mice show challenges regarding the ambiguous ejaculation timing. Here, we established a method for a mating environment with exact ejaculation timing. We also created a simple method for collecting pre- and post-ejaculatory uterine fluid without using forceps. Our methods achieved time-dependent biochemical and histological analyses of uterine fluids to provide fundamental information regarding protein composition and uterine structure changes during pre- and post-ejaculation. This protocol is suitable for analyzing temporal changes in reproductive phenomena, thereby contributing to elucidating the physiological role of the uterus in the process of intrauterine fertilization. Key features • This protocol is used for the simple collection of pre- and post-ejaculatory uterine fluid. • Changes in the pre- and post-ejaculatory intrauterine environment can be examined by controlling the dissection time of females after ejaculation. • An estrous female can be determined without a vaginal smear test in this protocol. • This protocol can be used to analyze the protein composition of post-ejaculatory uterine fluid and is applicable to analyze sperm within the uterus post-ejaculation.

    DOI: 10.21769/BioProtoc.5544

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  • Matrix stiffness regulates Mkx expression in rat tenocyte through TRPM7. 査読 国際誌

    Yuta Tsuchiya, Hikaru Matsuo, Hiroshi Asahara, Masafumi Inui

    Biochemistry and biophysics reports   43   102178 - 102178   2025年9月

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    担当区分:最終著者, 責任著者   記述言語:英語   掲載種別:研究論文(学術雑誌)  

    Tendon is the fibrous tissue that connects skeletal muscle and bone, playing a crucial role in transmitting forces generated in muscles to bones and thereby facilitating locomotion. Tendon is continuously subjected to mechanical stimuli, such as tensile force and shear stress, and it is well documented that tendon cells respond to these forces and modulate gene expression and tissue structures. However, whether or how tenocytes respond to matrix stiffness, another key mechanical cue for the tissue, remained elusive. While previous studies have shown that mesenchymal stem cells (MSCs) or tendon derived stem cells (TDSCs) modulate tenogenic gene expression in response to stiffness, its effect on tendon fibroblasts was unclear. In this study, we investigated the role of matrix stiffness on tenocytes derived from tail and Achilles tendon of young rats. Tenocytes displayed stiffness-dependent difference in expression of key tendon-related genes, including Mkx, particularly at 40 kPa stiffness. Interestingly, the transient receptor potential melastatin 7 (TRPM7) channel was identified as an upstream regulator of stiffness-dependent Mkx expression. TRPM7 expression was elevated at 40 kPa stiffness, and its knockdown reduced Mkx expression while abolishing the stiffness-dependent expression pattern. This regulation likely occurs through intracellular calcium (Ca2+) and/or magnesium (Mg2+) ion influx, as Mkx expression was promoted upon Ca2+ ionophore treatment or elevation of extracellular Mg2+ concentration. This study underscores the importance of stiffness in tendon biology and adds a novel layer to the transcriptional regulation of Mkx, with implications for understanding tendon development, maintenance, and mechanotransduction.

    DOI: 10.1016/j.bbrep.2025.102178

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  • Dynamic interactions between cartilaginous and tendinous/ligamentous primordia during musculoskeletal integration. 査読 国際誌

    Xinyi Yu, Ryosuke Kawakami, Shinsei Yambe, Yuki Yoshimoto, Takako Sasaki, Shinnosuke Higuchi, Hitomi Watanabe, Haruhiko Akiyama, Shigenori Miura, Kadi Hu, Gen Kondoh, Ramu Sagasaki, Masafumi Inui, Taiji Adachi, Denitsa Docheva, Takeshi Imamura, Chisa Shukunami

    Development (Cambridge, England)   152 ( 6 )   2025年3月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    Proper connections between cartilaginous and muscular primordia through tendinous/ligamentous primordia are essential for musculoskeletal integration. Herein, we report a novel double-reporter mouse model for investigating this process via fluorescently visualising scleraxis (Scx) and SRY-box containing gene 9 (Sox9) expression. We generated ScxTomato transgenic mice and crossed them with Sox9EGFP knock-in mice to obtain ScxTomato;Sox9EGFP mice. Deep imaging of optically cleared double-reporter embryos at E13.5 and E16.5 revealed previously unknown differences in the dynamic interactions between cartilaginous and tendinous/ligamentous primordia in control and Scx-deficient mice. Tendon/ligament maturation was evaluated through simultaneous detection of fluorescence and visualisation of collagen fibre formation using second harmonic generation imaging. Lack of deltoid tuberosity in Scx-deficient mice caused misdirected muscle attachment with morphological changes. Loss of Scx also dysregulated progenitor cell fate determination in the chondrotendinous junction, resulting in the formation of a rounded enthesis rather than the protruding enthesis observed in the control. Hence, our double-reporter mouse system, in combination with loss- or gain-of-function approaches, is a unique and powerful tool that could be used to gain a comprehensive understanding of musculoskeletal integration.

    DOI: 10.1242/dev.204512

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  • Complement Factor B Deficiency Is Dispensable for Female Fertility but Affects Microbiome Diversity and Complement Activity. 査読 国際誌

    Manato Sunamoto, Kazunori Morohoshi, Ban Sato, Ryo Mihashi, Masafumi Inui, Mitsutoshi Yamada, Kenji Miyado, Natsuko Kawano

    International journal of molecular sciences   26 ( 3 )   2025年2月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    Complement factor B (CFB) is a crucial component for the activation of the alternative pathway due to the formation of the C3 convertase with C3b, which further produces C3b to enhance the overall complement activity. Although Cfb is expressed not only in the immune tissues, but also in the reproductive tract, the physiological role of the alternative complement pathway in reproduction remains unclear. In this study, we addressed this issue by producing Cfb-knockout (KO) mice and analyzing their phenotypes. Sperm function, number of ovulated oocytes, and litter size were normal in KO mice. In contrast, the diversity of microbiomes in the gut and vaginal tract significantly increased in KO mice. Some serine protease activity in the serum from KO mice was lower than that of wild-type mice. Since the serum from KO mice showed significantly lower activity of the alternative complement pathway, CFB was found to be essential for this pathway. Our results indicate that although the alternative pathway is dispensable for normal fertility and development, it maintains the gut and vaginal microbiomes by suppressing their diversity and activating the alternative complement pathway.

    DOI: 10.3390/ijms26031393

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  • Dynamics of post-ejaculated intrauterine environment in mice. 国際誌

    Yu Matsumoto, Ban Sato, Masafumi Inui, Natsuko Kawano, Kenji Miyado

    microPublication biology   2025   2025年

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    After ejaculation, the intrauterine environment undergoes dynamic fluid changes due to post-ejaculated uterine fluid (eUF) coagulation and subsequent liquefaction. These changes presumably contribute to fertilization and reproductive efficiency; however, their physiological roles remain unclear. We studied the significance of the post-ejaculated intrauterine environment during in vivo fertilization. eUF coagulated immediately after ejaculation, and histological analysis of the uterus suggested that eUF liquefaction was promoted 6-10 h post-ejaculation. However, most gametes completed fertilization within 4 h post-ejaculation. Since eUF fluid changes did not align with fertilization timing, they are assumed to contribute to reproductive phenomena beyond sperm transport and release.

    DOI: 10.17912/micropub.biology.001872

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  • Epigenome editing revealed the role of DNA methylation of T-DMR/CpG island shore on Runx2 transcription. 査読 国際誌

    Yutaro Kawa, Miyuki Shindo, Jun Ohgane, Masafumi Inui

    Biochemistry and biophysics reports   38   101733 - 101733   2024年7月

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    担当区分:最終著者, 責任著者   記述言語:英語   掲載種別:研究論文(学術雑誌)  

    RUNX2 is a transcription factor crucial for bone formation. Mutant mice with varying levels of Runx2 expression display dosage-dependent skeletal abnormalities, underscoring the importance of Runx2 dosage control in skeletal formation. RUNX2 activity is regulated by several molecular mechanisms, including epigenetic modification such as DNA methylation. In this study, we investigated whether targeted repressive epigenome editing including hypermethylation to the Runx2-DMR/CpG island shore could influence Runx2 expression using Cas9-based epigenome-editing tools. Through the transient introduction of CRISPRoff-v2.1 and gRNAs targeting Runx2-DMR into MC3T3-E1 cells, we successfully induced hypermethylation of the region and concurrently reduced Runx2 expression during osteoblast differentiation. Although the epigenome editing of Runx2-DMR did not impact the expression of RUNX2 downstream target genes, these results indicate a causal relationship between the epigenetic status of the Runx2-DMR and Runx2 transcription. Additionally, we observed that hypermethylation of the Runx2-DMR persisted for at least 24 days under growth conditions but decreased during osteogenic differentiation, highlighting an endogenous DNA demethylation activity targeting the Runx2-DMR during the differentiation process. In summary, our study underscore the usefulness of the epigenome editing technology to evaluate the function of endogenous genetic elements and revealed that the Runx2-DMR methylation is actively regulated during osteoblast differentiation, subsequently could influence Runx2 expression.

    DOI: 10.1016/j.bbrep.2024.101733

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  • Automated xeno-free chondrogenic differentiation from human embryonic stem cells: Enhancing efficiency and ensuring high-quality mass production 査読

    Jun Long Chen, Oki Kataoka, Kazeto Tsuchiya, Yoshie Oishi, Ayumi Takao, Yen Chih Huang, Hiroko Komura, Saeko Akiyama, Ren Itou, Masafumi Inui, Shin Enosawa, Hidenori Akutsu, Makoto Komura, Yasushi Fuchimoto, Akihiro Umezawa

    Regenerative Therapy   26   889 - 900   2024年6月

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    掲載種別:研究論文(学術雑誌)  

    DOI: 10.1016/j.reth.2024.09.007

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  • Scleraxis-lineage cells are required for correct muscle patterning. 査読 国際誌

    Yudai Ono, Saundra Schlesinger, Kanako Fukunaga, Shinsei Yambe, Tempei Sato, Takako Sasaki, Chisa Shukunami, Hiroshi Asahara, Masafumi Inui

    Development (Cambridge, England)   150 ( 10 )   2023年5月

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    担当区分:最終著者, 責任著者   記述言語:英語   掲載種別:研究論文(学術雑誌)  

    Movement of the vertebrate body is supported by the connection of muscle, tendon and bone. Each skeletal muscle in the vertebrate body has a unique shape and attachment site; however, the mechanism that ensures reproducible muscle patterning is incompletely understood. In this study, we conducted targeted cell ablation using scleraxis (Scx)-Cre to examine the role of Scx-lineage cells in muscle morphogenesis and attachment in mouse embryos. We found that muscle bundle shapes and attachment sites were significantly altered in embryos with Scx-lineage cell ablation. Muscles in the forelimb showed impaired bundle separation and limb girdle muscles distally dislocated from their insertion sites. Scx-lineage cells were required for post-fusion myofiber morphology, but not for the initial segregation of myoblasts in the limb bud. Furthermore, muscles could change their attachment site, even after formation of the insertion. Lineage tracing suggested that the muscle patterning defect was primarily attributed to the reduction of tendon/ligament cells. Our study demonstrates an essential role of Scx-lineage cells in the reproducibility of skeletal muscle attachment, in turn revealing a previously unappreciated tissue-tissue interaction in musculoskeletal morphogenesis.

    DOI: 10.1242/dev.201101

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  • Simultaneous loss of skeletal muscle myosin heavy chain IIx and IIb causes severe skeletal muscle hypoplasia in postnatal mice. 査読 国際誌

    Keisuke Hitachi, Yuri Kiyofuji, Hisateru Yamaguchi, Masashi Nakatani, Masafumi Inui, Kunihiro Tsuchida

    FASEB journal : official publication of the Federation of American Societies for Experimental Biology   37 ( 1 )   e22692   2023年1月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    The skeletal muscle myosin heavy chain (MyHC) is a fundamental component of the sarcomere structure and muscle contraction. Two of the three adult fast MyHCs, MyHC-IIx and MyHC-IIb, are encoded by Myh1 and Myh4, respectively. However, skeletal muscle disorders have not yet been linked to these genes in humans. MyHC-IIb is barely detectable in human skeletal muscles. Thus, to characterize the molecular function of skeletal muscle MyHCs in humans, investigation of the effect of simultaneous loss of MyHC-IIb and other MyHCs on skeletal muscle in mice is essential. Here, we generated double knockout (dKO) mice with simultaneous loss of adult fast MyHCs by introducing nonsense frameshift mutations into the Myh1 and Myh4 genes. The dKO mice appeared normal after birth and until 2 weeks of age but showed severe skeletal muscle hypoplasia after 2 weeks. In 3-week-old dKO mice, increased expression of other skeletal muscle MyHCs, such as MyHC-I, MyHC-IIa, MyHC-neo, and MyHC-emb, was observed. However, these expressions were not sufficient to compensate for the loss of MyHC-IIb and MyHC-IIx. Moreover, the aberrant sarcomere structure with altered expression of sarcomere components was observed in dKO mice. Our findings imply that the simultaneous loss of MyHC-IIb and MyHC-IIx is substantially detrimental to postnatal skeletal muscle function and will contribute to elucidating the molecular mechanisms of skeletal muscle wasting disorders caused by the loss of skeletal muscle MyHCs.

    DOI: 10.1096/fj.202200581R

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  • Digoxigenin-labeled RNA probes for untranslated regions enable the isoform-specific gene expression analysis of myosin heavy chains in whole-mount in situ hybridization. 査読

    Masafumi Tanji, Keitaro Wada, Keita Sakamoto, Yudai Ono, Masafumi Inui

    Development, growth & differentiation   2022年12月

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    担当区分:最終著者, 責任著者   記述言語:英語   掲載種別:研究論文(学術雑誌)  

    Myosin heavy chains (MyHCs), which are encoded by myosin heavy chain (Myh) genes, are the most abundant proteins in myofiber. Among the 11 sarcomeric Myh isoform genes in the mammalian genome, 7 are mainly expressed in skeletal muscle. Myh genes/MyHC proteins share a common role as force producing units with highly conserved sequences, but have distinct spatio-temporal expression patterns. As such, the expression patterns of Myh genes/MyHC proteins are considered as molecular signatures of specific fiber types or the regenerative status of mammalian skeletal muscles. Immunohistochemistry is widely used for identifying MyHC expression patterns; however, this method is costly and is not ideal for whole-mount samples, such as embryos. In situ hybridization (ISH) is another versatile method for the analysis of gene expression, but is not commonly applied for Myh genes, partly because of the highly homologous sequences of Myh genes. Here we demonstrate that an ISH analysis with the untranslated region (UTR) sequence of Myh genes is cost-effective and specific method for analyzing the Myh gene expression in whole-mount samples. Digoxigenin (DIG)-labeled antisense probes for UTR sequences, but not for protein coding sequences, specifically detected the expression patterns of respective Myh isoform genes in both embryo and adult skeletal muscle tissues. UTR probes also revealed the isoform gene-specific polarized localization of Myh mRNAs in embryonic myofibers, which implied a novel mRNA distribution mechanism. Our data suggested that the DIG-labeled UTR probe is a cost-effective and versatile method to specifically detect skeletal muscle Myh genes in a whole-mount analysis.

    DOI: 10.1111/dgd.12832

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  • Myh1とMyh4遺伝子の同時欠損による骨格筋機能への影響の解析

    常陸 圭介, 清藤 友梨, 山口 央輝, 中谷 直史, 乾 雅史, 土田 邦博

    日本筋学会学術集会プログラム・抄録集   8回   88 - 88   2022年8月

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    記述言語:日本語   出版者・発行元:(一社)日本筋学会  

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  • Protocadherin-1 is expressed in the notochord of mouse embryo but is dispensable for its formation. 査読 国際誌

    Kanako Fukunaga, Masafumi Tanji, Nana Hanzawa, Hiroki Kuroda, Masafumi Inui

    Biochemistry and biophysics reports   27   101047 - 101047   2021年9月

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    担当区分:最終著者, 責任著者   記述言語:英語   掲載種別:研究論文(学術雑誌)  

    Notochord is an embryonic midline structure that serves as mechanical support for axis elongation and the signaling center for the surrounding tissues. Precursors of notochord are initially induced in the dorsal most mesoderm region in gastrulating embryo and separate from the surrounding mesoderm/endoderm tissue to form an elongated rod-like structure, suggesting that cell adhesion molecules may play an important role in this step. In Xenopus embryo, axial protocadherin (AXPC), an orthologue of mammalian Protocadherin-1 (PCDH1), is indispensable for the assembly and separation from the surrounding tissue of the notochord cells. However, the role of PCDH1 in mammalian notochord remains unknown. We herein report that PCDH1 is expressed in the notochord of mouse embryo and that PCDH1-deficient mice form notochord normally. First, we examined the temporal expression pattern of pcdh1 and found that pcdh1 mRNA was expressed from embryonic day (E) 7.5, prior to the stage when notochord cells detach from the surrounding endoderm tissue. Second, we found that PCDH1 protein is expressed in the notochord of mouse embryos in addition to the previously reported expression in endothelial cells. To further investigate the role of PCDH1 in embryonic development, we generated PCDH1-deficient mice using the CRISPR-Cas9 system. In PCDH1-deficient embryos, notochord formation and separation from the surrounding tissue were normal. Structure and marker gene expression of notochord were also unaffected by loss of PCDH1. Major vascular patterns in PCDH1-deficient embryo were essentially normal. These results suggest that PCDH1 is dispensable for notochord formation, including the tissue separation process, in mammalian embryos. We successfully identified the evolutionary conserved expression of PCDH1 in notochord, but its function may differ among species.

    DOI: 10.1016/j.bbrep.2021.101047

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  • Lin28a/let-7 pathway modulates the Hox code via Polycomb regulation during axial patterning in vertebrates. 査読 国際誌

    Tempei Sato, Kensuke Kataoka, Yoshiaki Ito, Shigetoshi Yokoyama, Masafumi Inui, Masaki Mori, Satoru Takahashi, Keiichi Akita, Shuji Takada, Hiroe Ueno-Kudoh, Hiroshi Asahara

    eLife   9   2020年5月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    The body plan along the anteroposterior axis and regional identities are specified by the spatiotemporal expression of Hox genes. Multistep controls are required for their unique expression patterns; however, the molecular mechanisms behind the tight control of Hox genes are not fully understood. In this study, we demonstrated that the Lin28a/let-7 pathway is critical for axial elongation. Lin28a-/- mice exhibited axial shortening with mild skeletal transformations of vertebrae, which were consistent with results in mice with tail bud-specific mutants of Lin28a. The accumulation of let-7 in Lin28a-/- mice resulted in the reduction of PRC1 occupancy at the Hox cluster loci by targeting Cbx2. Consistently, Lin28a loss in embryonic stem-like cells led to aberrant induction of posterior Hox genes, which was rescued by the knockdown of let-7. These results suggest that the Lin28/let-7 pathway is involved in the modulation of the 'Hox code' via Polycomb regulation during axial patterning.

    DOI: 10.7554/eLife.53608

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  • Generation of a Quantitative Luciferase Reporter for Sox9 SUMOylation. 査読 国際誌

    Hideka Saotome, Atsumi Ito, Atsushi Kubo, Masafumi Inui

    International journal of molecular sciences   21 ( 4 )   2020年2月

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    担当区分:最終著者, 責任著者   記述言語:英語  

    Sox9 is a master transcription factor for chondrogenesis, which is essential for chondrocyte proliferation, differentiation, and maintenance. Sox9 activity is regulated by multiple layers, including post-translational modifications, such as SUMOylation. A detection method for visualizing the SUMOylation in live cells is required to fully understand the role of Sox9 SUMOylation. In this study, we generated a quantitative reporter for Sox9 SUMOylation that is based on the NanoBiT system. The simultaneous expression of Sox9 and SUMO1 constructs that are conjugated with NanoBiT fragments in HEK293T cells induced luciferase activity in SUMOylation target residue of Sox9-dependent manner. Furthermore, the reporter signal could be detected from both cell lysates and live cells. The signal level of our reporter responded to the co-expression of SUMOylation or deSUMOylation enzymes by several fold, showing dynamic potency of the reporter. The reporter was active in multiple cell types, including ATDC5 cells, which have chondrogenic potential. Finally, using this reporter, we revealed a extracellular signal conditions that can increase the amount of SUMOylated Sox9. In summary, we generated a novel reporter that was capable of quantitatively visualizing the Sox9-SUMOylation level in live cells. This reporter will be useful for understanding the dynamism of Sox9 regulation during chondrogenesis.

    DOI: 10.3390/ijms21041274

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  • Deletion of a Seminal Gene Cluster Reinforces a Crucial Role of SVS2 in Male Fertility. 査読 国際誌

    Miyuki Shindo, Masafumi Inui, Woojin Kang, Moe Tamano, Cai Tingwei, Shuji Takada, Taku Hibino, Manabu Yoshida, Kaoru Yoshida, Hiroshi Okada, Teruaki Iwamoto, Kenji Miyado, Natsuko Kawano

    International journal of molecular sciences   20 ( 18 )   4557   2019年9月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    Multiple genes, whose functions or expression are overlapping, compensate for the loss of one gene. A gene cluster in the mouse genome encodes five seminal vesicle proteins (SVS2, SVS3, SVS4, SVS5, and SVS6). These proteins are produced by male rodents and function in formation of the copulatory plug following mating. SVS2 plays an essential role in the successful internal fertilization by protecting the sperm membrane against a uterine immune attack. We hypothesized that the four remaining seminal vesicle proteins (SVPs) of this gene cluster may partially/completely compensate for the deficiency of SVS2. For confirming our hypothesis, we generated mice lacking the entire SVP-encoding gene cluster and compared their fecundity with Svs2-deficient (Svs2-/-) mice; that is, mice deficient in Svs2 alone. A single loxP site remained after the deletion of the Svs2 gene. Therefore, we inserted another loxP site by combining the CRISPR/Cas9 system with single-stranded oligodeoxynucleotides (ssODN). Male mice lacking the entire SVP-encoding gene cluster (Svs2-6-/- mice) and thereby all five SVP proteins, generated by the deletion of 100kbp genomic DNA, showed low fecundity. However, the fecundity level was comparable with that from Svs2-/- male mice. Our results demonstrate that SVS3, SVS4, SVS5, and SVS6 do not function in the protection of sperm against a uterine immune attack in the absence of SVS2. Thus, Svs2 is the critical gene in the SVP gene cluster.

    DOI: 10.3390/ijms20184557

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    その他リンク: http://orcid.org/0000-0003-4720-007X

  • Comparative analysis demonstrates cell type-specific conservation of SOX9 targets between mouse and chicken. 査読 国際誌

    Satoshi Yamashita, Kensuke Kataoka, Hiroto Yamamoto, Tomoko Kato, Satoshi Hara, Katsushi Yamaguchi, Claire Renard-Guillet, Yuki Katou, Katsuhiko Shirahige, Haruki Ochi, Hajime Ogino, Tokujiro Uchida, Masafumi Inui, Shuji Takada, Shuji Shigenobu, Hiroshi Asahara

    Scientific reports   9 ( 1 )   12560 - 12560   2019年8月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    SRY (sex-determining region Y)-box 9 (SOX9) is a transcription factor regulating both chondrogenesis and sex determination. Among vertebrates, SOX9's functions in chondrogenesis are well conserved, while they vary in sex determination. To investigate the conservation of SOX9's regulatory functions in chondrogenesis and gonad development among species, we performed chromatin immunoprecipitation sequencing (ChIP-seq) using developing limb buds and male gonads from embryos of two vertebrates, mouse and chicken. In both mouse and chicken, SOX9 bound to intronic and distal regions of genes more frequently in limb buds than in male gonads, while SOX9 bound to the proximal upstream regions of genes more frequently in male gonads than in limb buds. In both species, SOX palindromic repeats were identified more frequently in SOX9 binding regions in limb bud genes compared with those in male gonad genes. The conservation of SOX9 binding regions was significantly higher in limb bud genes. In addition, we combined RNA expression analysis (RNA sequencing) with the ChIP-seq results at the same stage in developing chondrocytes and Sertoli cells and determined SOX9 target genes in these cells of the two species and disclosed that SOX9 targets showed high similarity of targets in chondrocytes, but not in Sertoli cells.

    DOI: 10.1038/s41598-019-48979-4

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  • Creation of CRISPR-based germline-genome-engineered mice without ex vivo handling of zygotes by i-GONAD. 査読 国際誌

    Gurumurthy CB, Sato M, Nakamura A, Inui M, Kawano N, Islam MA, Ogiwara S, Takabayashi S, Matsuyama M, Nakagawa S, Miura H, Ohtsuka M

    Nature protocols   14 ( 8 )   2452 - 2482   2019年7月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1038/s41596-019-0187-x

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  • Wwp2 maintains cartilage homeostasis through regulation of Adamts5. 査読 国際誌

    Mokuda S, Nakamichi R, Matsuzaki T, Ito Y, Sato T, Miyata K, Inui M, Olmer M, Sugiyama E, Lotz M, Asahara H

    Nature communications   10 ( 1 )   2429 - 2429   2019年6月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1038/s41467-019-10177-1

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  • Dissecting the roles of miR-140 and its host gene 査読

    Masafumi Inui, Sho Mokuda, Tempei Sato, Moe Tamano, Shuji Takada, Hiroshi Asahara

    Nature Cell Biology   20 ( 5 )   516 - 518   2018年5月

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    担当区分:筆頭著者, 責任著者   記述言語:英語   出版者・発行元:Nature Publishing Group  

    DOI: 10.1038/s41556-018-0077-4

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  • Tendons and Ligaments: Connecting Developmental Biology to Musculoskeletal Disease Pathogenesis 査読

    Hiroshi Asahara, Masafumi Inui, Martin K. Lotz

    JOURNAL OF BONE AND MINERAL RESEARCH   32 ( 9 )   1773 - 1782   2017年9月

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    担当区分:責任著者   記述言語:英語  

    DOI: 10.1002/jbmr.3199

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  • CRISPR/Cas9-mediated simultaneous knockout of Dmrt1 and Dmrt3 does not recapitulate the 46,XY gonadal dysgenesis observed in 9p24.3 deletion patients 査読

    Masafumi Inui, Moe Tamano, Tomoko Kato, Shuji Takada

    Biochemistry and Biophysics Reports   9   238 - 244   2017年3月

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    担当区分:筆頭著者, 責任著者   記述言語:英語   掲載種別:研究論文(学術雑誌)   出版者・発行元:Elsevier B.V.  

    DOI: 10.1016/j.bbrep.2017.01.001

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  • NR5A1ミスセンス変異p.R92Wは、ヒトとマウスに共通する46,XY精巣形成不全とヒト特異的46,XX精巣形成を招く 査読

    宮戸 真美, 乾 雅史, 五十嵐 麻希, 福井 由宇子, 玉野 萌恵, 宮戸 健二, 緒方 勤, 高田 修治, 深見 真紀

    日本内分泌学会雑誌   92 ( 3 )   833 - 833   2017年1月

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    記述言語:日本語   出版者・発行元:(一社)日本内分泌学会  

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  • The p.R92W variant of NR5A1/Nr5a1 induces testicular development of 46,XX gonads in humans, but not in mice: phenotypic comparison of human patients and mutation-induced mice 査読

    Mami Miyado, Masafumi Inui, Maki Igarashi, Yuko Katoh-Fukui, Kei Takasawa, Akiko Hakoda, Junko Kanno, Kenichi Kashimada, Kenji Miyado, Moe Tamano, Tsutomu Ogata, Shuji Takada, Maki Fukami

    BIOLOGY OF SEX DIFFERENCES   7   56   2016年11月

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  • Mohawk promotes the maintenance and regeneration of the outer annulus fibrosus of intervertebral discs 査読

    Ryo Nakamichi, Yoshiaki Ito, Masafumi Inui, Naoko Onizuka, Tomohiro Kayama, Kensuke Kataoka, Hidetsugu Suzuki, Masaki Mori, Masayo Inagawa, Shizuko Ichinose, Martin K. Lotz, Daisuke Sakai, Koichi Masuda, Toshifumi Ozaki, Hiroshi Asahara

    NATURE COMMUNICATIONS   7   12503   2016年8月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1038/ncomms12503

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  • Generation of mutant mice via the CRISPR/Cas9 system using FokI-dCas9 査読

    Satoshi Hara, Moe Tamano, Satoshi Yamashita, Tomoko Kato, Takeshi Saito, Tetsushi Sakuma, Takashi Yamamoto, Masafumi Inui, Shuji Takada

    SCIENTIFIC REPORTS   5   11221   2015年6月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1038/srep11221

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  • Transcription Factor Mohawk Controls Tenogenic Differentiation of Bone Marrow Mesenchymal Stem Cells In Vitro and In Vivo 査読

    Koji Otabe, Hiroyuki Nakahara, Akihiko Hasegawa, Tetsuya Matsukawa, Fumiaki Ayabe, Naoko Onizuka, Masafumi Inui, Shuji Takada, Yoshiaki Ito, Ichiro Sekiya, Takeshi Muneta, Martin Lotz, Hiroshi Asahara

    JOURNAL OF ORTHOPAEDIC RESEARCH   33 ( 1 )   1 - 8   2015年1月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1002/jor.22750

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  • Transcription factor Mohawk controls tenogenic differentiation of bone marrow mesenchymal stem cells in vitro and in vivo. 国際誌

    Koji Otabe, Hiroyuki Nakahara, Akihiko Hasegawa, Tetsuya Matsukawa, Fumiaki Ayabe, Naoko Onizuka, Masafumi Inui, Shuji Takada, Yoshiaki Ito, Ichiro Sekiya, Takeshi Muneta, Martin Lotz, Hiroshi Asahara

    Journal of orthopaedic research : official publication of the Orthopaedic Research Society   33 ( 1 )   1 - 8   2015年1月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    Mohawk homeobox (MKX) has been demonstrated as a tendon/ligament specific transcription factor. The aim of this study was to investigate the role of MKX in ligament/tenogenic differentiation of bone marrow derived mesenchymal stem cells (BMMSCs). Human BMMSCs were treated with 50 ng/ml BMP-12 or transduced with MKX or scleraxis (SCX) adenoviral vector. Gene expression analysis was performed by quantitative reverse transcribed polymerase chain reaction (qRT-PCR). Rat BMMSCs were seeded in a collagen scaffold and transplanted into a rat Achilles tendon defect model. Tenogenesis related gene expressions and histological features were analyzed. BMP-12 induced tenogenesis in BMMSCs as indicated by increased COL1a1, TNXB, DCN and SCX mRNA, and MKX expression increased simultaneously. Rat BMMSCs enhanced defect repair and were still detectable 3 weeks after transplantation. Increased expressions of COL1a1, TNC and TNMD in vivo were also correlated with upregulated MKX. Adenoviral MKX promoted expression of COL1a1, TNXB, and TNMD in BMMSCs. This study demonstrated that MKX gene expression is enhanced during the tenogenic differentiation of BMMSCs in vitro and in vivo, and the adenoviral overexpression of MKX increases tendon extracellular matrix gene expression and protein production. Thus, MKX is a key factor for tenogenic differentiation of MSCs.

    DOI: 10.1002/jor.22750

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  • Rapid generation of mouse models with defined point mutations by the CRISPR/Cas9 system 査読

    Masafumi Inui, Mami Miyado, Maki Igarashi, Moe Tamano, Atsushi Kubo, Satoshi Yamashita, Hiroshi Asahara, Maki Fukami, Shuji Takada

    SCIENTIFIC REPORTS   4   5396   2014年6月

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    担当区分:筆頭著者, 責任著者   記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1038/srep05396

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  • Production of Sry knockout mouse using TALEN via oocyte injection 査読

    Tomoko Kato, Kohei Miyata, Miku Sonobe, Satoshi Yamashita, Moe Tamano, Kento Miura, Yoshiakira Kanai, Shingo Miyamoto, Tetsushi Sakuma, Takashi Yamamoto, Masafumi Inui, Takefumi Kikusui, Hiroshi Asahara, Shuji Takada

    Scientific Reports   3   3136   2013年11月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1038/srep03136

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  • Signaling crosstalk between TGFβ and Dishevelled/Par1b. 国際誌

    A Mamidi, M Inui, A Manfrin, S Soligo, E Enzo, M Aragona, M Cordenonsi, O Wessely, S Dupont, S Piccolo

    Cell death and differentiation   19 ( 10 )   1689 - 97   2012年10月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    Crosstalk of signaling pathways is critical during metazoan development and adult tissue homeostasis. Even though the transforming growth factor-beta (TGFβ) transduction cascade is rather simple, in vivo responsiveness to TGFβ ligands is tightly regulated at several steps. As such, TGFβ represents a paradigm for how the activity of one signaling system is modulated by others. Here, we report an unsuspected regulatory step involving Dishevelled (Dvl) and Par1b (also known as MARK2). Dvl and Par1b cooperate to enable TGFβ/bone morphogenetic protein (BMP) signaling in Xenopus mesoderm development and TGFβ responsiveness in mammalian cells. Mechanistically, the assembly of the Par1b/Dvl3/Smad4 complex is fostered by Wnt5a. The association of Smad4 to Dvl/Par1 prevents its inhibitory ubiquitination by ectodermin (also known as transcriptional intermediary factor 1 gamma or tripartite motif protein 33). We propose that this crosstalk is relevant to coordinate TGFβ responses with Wnt-noncanonical and polarity pathways.

    DOI: 10.1038/cdd.2012.50

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  • Self-regulation of the head-inducing properties of the Spemann organizer 査読

    Masafumi Inui, Marco Montagner, Danny Ben-Zvi, Graziano Martello, Sandra Soligo, Andrea Manfrin, Mariaceleste Aragona, Elena Enzo, Luca Zacchigna, Francesca Zanconato, Luca Azzolin, Sirio Dupont, Michelangelo Cordenonsi, Stefano Piccolo

    PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA   109 ( 38 )   15354 - 15359   2012年9月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1073/pnas.1203000109

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  • Regulation of TGF-β signal transduction by mono- and deubiquitylation of Smads. 査読

    Dupont S, Inui M, Newfeld SJ

    FEBS letters   586 ( 14 )   1913 - 1920   2012年7月

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  • miRNAs and morphogen gradients. 査読

    Inui M, Montagner M, Piccolo S

    Current opinion in cell biology   24 ( 2 )   194 - 201   2012年4月

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  • USP15 is a deubiquitylating enzyme for receptor-activated SMADs 査読

    Masafumi Inui, Andrea Manfrin, Anant Mamidi, Graziano Martello, Leonardo Morsut, Sandra Soligo, Elena Enzo, Stefano Moro, Simona Polo, Sirio Dupont, Michelangelo Cordenonsi, Stefano Piccolo

    NATURE CELL BIOLOGY   13 ( 11 )   1368 - U187   2011年11月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1038/ncb2346

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  • The Hippo Transducer TAZ Confers Cancer Stem Cell-Related Traits on Breast Cancer Cells 査読

    Michelangelo Cordenonsi, Francesca Zanconato, Luca Azzolin, Mattia Forcato, Antonio Rosato, Chiara Frasson, Masafumi Inui, Marco Montagner, Anna R. Parenti, Alessandro Poletti, Maria Grazia Daidone, Sirio Dupont, Giuseppe Basso, Silvio Bicciato, Stefano Piccolo

    CELL   147 ( 4 )   759 - 772   2011年11月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1016/j.cell.2011.09.048

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  • An in vitro reconstitution system for the assessment of chromatin protein fluidity during Xenopus development 査読

    Ryuta Aoki, Masafumi Inui, Yohei Hayashi, Ayako Sedohara, Koji Okabayashi, Kiyoshi Ohnuma, Masayuki Murata, Makoto Asashima

    BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS   400 ( 2 )   200 - 206   2010年9月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1016/j.bbrc.2010.08.032

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  • MicroRNA control of signal transduction 査読

    Masafumi Inui, Graziano Martello, Stefano Piccolo

    NATURE REVIEWS MOLECULAR CELL BIOLOGY   11 ( 4 )   252 - 263   2010年4月

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  • FAM/USP9x, a Deubiquitinating Enzyme Essential for TGF beta Signaling, Controls Smad4 Monoubiquitination 査読

    Sirio Dupont, Anant Mamidi, Michelangelo Cordenonsi, Marco Montagner, Luca Zacchigna, Maddalena Adorno, Graziano Martello, Michael J. Stinchfield, Sandra Soligo, Leonardo Morsut, Masafumi Inui, Stefano Moro, Nicola Modena, Francesco Argenton, Stuart J. Newfeld, Stefano Piccolo

    CELL   136 ( 1 )   123 - 135   2009年1月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1016/j.cell.2008.10.051

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  • Tbx6, Thylacine1, and E47 synergistically activate bowline expression in Xenopus somitogenesis 査読

    Keisuke Hitachi, Akiko Kondow, Hiroki Danno, Masafumi Inui, Hideho Uchiyama, Makoto Asashima

    DEVELOPMENTAL BIOLOGY   313 ( 2 )   816 - 828   2008年1月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1016/j.ydbio.2007.10.015

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  • MicroRNA control of nodal signalling 査読

    Graziano Martello, Luca Zacchigna, Masafumi Inui, Marco Montagner, Maddalena Adorno, Anant Mamidi, Leonardo Morsut, Sandra Soligo, Uyen Tran, Sirio Dupont, Michelangelo Cordenonsi, Oliver Wessely, Stefano Piccolo

    NATURE   449 ( 7159 )   183 - U1   2007年9月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1038/nature06100

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  • TSC-box is essential for the nuclear localization and antiproliferative effect of XTSC-22 査読

    Akiko Hashiguchi, Keisuke Hitachi, Masafumi Inui, Koji Okabayashi, Makoto Asashima

    DEVELOPMENT GROWTH & DIFFERENTIATION   49 ( 3 )   197 - 204   2007年4月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1111/j.1440-169x.2007.00908.x

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  • A novel gene, BENI is required for the convergent extension during Xenopus laevis gastrulation 査読

    Motohiro Homma, Masafumi Inui, Akimasa Fukui, Tatsuo Michiue, Koji Okabayashi, Makoto Asashima

    DEVELOPMENTAL BIOLOGY   303 ( 1 )   270 - 280   2007年3月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1016/j.ydbio.2006.11.014

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  • Xapelin and Xmsr are required for cardiovascular development in Xenopus laevis 査読

    Masafumi Inui, Akimasa Fukui, Yuzuru Ito, Makoto Asashima

    DEVELOPMENTAL BIOLOGY   298 ( 1 )   188 - 200   2006年10月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1016/j.ydbio.2006.06.028

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  • A novel gene, Ami is expressed in vascular tissue in Xenopus laevis 査読

    M Inui, M Asashima

    GENE EXPRESSION PATTERNS   6 ( 6 )   613 - 619   2006年8月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1016/j.modgep.2005.11.014

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  • Identification and characterization of Xenopus OMP25 査読

    M Inui, M Asashima

    DEVELOPMENT GROWTH & DIFFERENTIATION   46 ( 5 )   405 - 412   2004年10月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1111/j.1440-169x.2004.00757.x

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  • Axial protocadherin is a mediator of prenotochord cell sorting in Xenopus 査読

    H Kuroda, M Inui, K Sugimoto, T Hayata, M Asashima

    DEVELOPMENTAL BIOLOGY   244 ( 2 )   267 - 277   2002年4月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    DOI: 10.1006/dbio.2002.0589

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  • Bacteriophage WO and virus-like particles in Wolbachia, an endosymbiont of arthropods. 国際誌

    S Masui, H Kuroiwa, T Sasaki, M Inui, T Kuroiwa, H Ishikawa

    Biochemical and biophysical research communications   283 ( 5 )   1099 - 104   2001年5月

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    記述言語:英語   掲載種別:研究論文(学術雑誌)  

    Wolbachia are intracellular symbionts mainly found in arthropods, causing various sexual alterations on their hosts by unknown mechanisms. Here we report the results that strongly suggest that Wolbachia have virus-like particles of phage WO, which was previously identified as a prophage-like element in the Wolbachia genome. Wolbachia (strain wTai) infection in an insect was detected with the antibody against Wsp, an outer surface protein of Wolbachia, by fluorescence microscopy and immunoelectron-microscopy for the first time. Virus-like particles in Wolbachia were observed by electron-microscopy. The 0.22-microm filtrate of insect ovary contained DAPI-positive particles, and PCR analysis demonstrated that a phage WO DNA passed through the filter while Wolbachia DNA were eliminated, suggesting that the DAPI-positive particles were phage WO.

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MISC

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共同研究・競争的資金等の研究課題

  • Sox9SUMO化を標的とした骨軟骨機能維持の試み

    研究課題/領域番号:24K22257  2024年6月 - 2027年3月

    日本学術振興会  科学研究費助成事業  挑戦的研究(萌芽)

    乾 雅史

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    配分額:6370000円 ( 直接経費:4900000円 、 間接経費:1470000円 )

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  • 再生・移植医療用細胞・組織構築物の非侵襲的品質評価法の確立

    研究課題/領域番号:23H03782  2023年4月 - 2027年3月

    日本学術振興会  科学研究費助成事業  基盤研究(B)

    宮本 義孝, 池内 真志, 乾 雅史, 河野 菜摘子, 中林 一彦

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    配分額:18590000円 ( 直接経費:14300000円 、 間接経費:4290000円 )

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  • 再生・移植医療用細胞・組織構築物の非侵襲的品質評価法の確立

    研究課題/領域番号:23K28470  2023年4月 - 2027年3月

    日本学術振興会  科学研究費助成事業  基盤研究(B)

    宮本 義孝, 池内 真志, 乾 雅史, 河野 菜摘子, 中林 一彦

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    配分額:18590000円 ( 直接経費:14300000円 、 間接経費:4290000円 )

    再生・移植医療用細胞・組織構築物の品質を非侵襲的に評価することを目的とする.再生・移植医療分野で,移植するための細胞・組織や再生医療等製品の品質を見極めることは,治療の成功率を高めるために極めて重要である.そこで,本研究では,移植前に,再生・移植医療用細胞・組織構築物の品質を判定する技術の確立を行う.具体的な研究課題として,①細胞・組織構築物の作製とOCTによる非侵襲的品質評価,②細胞・組織シートの作製とTEER評価,③培養骨格筋組織の作製と電気刺激評価,について検討した.
    本年度(1年目)における各研究課題に対する主な成果をまとめた.①本研究では,3D培養デバイスを用いて,細胞・組織構築物を調製した.OCTによる細胞・組織構築物の3D画像を取得し,非侵襲的な品質評価を検討した.②本研究では,A549細胞(ヒト肺胞上皮癌由来細胞)およびHH細胞(ウシ由来頸動脈正常血管内皮細胞)を用いて,それぞれの細胞単層膜を作製し,細胞バリア機能を評価した.また,特長の異なる磁性ナノ微粒子を暴露することで,それぞれの細胞単層膜に与える影響を検討した.TEER測定の結果,磁性ナノ微粒子の有無で有意差は見られず,細胞バリア機能が維持されていることがわかった.③本研究では,ポリジメチルシロキサン(PDMS)で作成したデバイスを用いて,培養骨格筋組織を作成し,電気刺激を与え,筋組織の収縮率,面積,輪の外周長,輪の内周長,の変化率を調べた.結果,デバイス内にピラーを用いることで,輪状に筋線維を配向させ,内径収縮率を向上することに成功した.
    以上より,本研究では、①②③で得られた成果をもとに,各々の非侵襲的評価法による細胞・組織構築物の品質評価に成功している.

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  • 腱を中心とした運動器形態形成メカニズムの解明

    研究課題/領域番号:23K23899  2022年4月 - 2025年3月

    日本学術振興会  科学研究費助成事業  基盤研究(B)

    乾 雅史

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    配分額:17680000円 ( 直接経費:13600000円 、 間接経費:4080000円 )

    脊椎動物の運動器は、骨格筋、骨、軟骨、そして骨格筋と骨軟骨をつなぐ腱により機能的な形態が構成されるが、その形成メカニズムの解明は 不十分である。本研究は腱を中心とした、組織間相互作用による形態形成メカニズムの解明を目的とし、1. 筋腱結合を誘導する因子の同定、2. noncoding RNAによる腱骨境界形成制御の解析、3. 腱前駆細胞を規定する転写因子Scxの発現制御や標的遺伝子の機能解析に取り組んでいる。2023年度は課題1筋腱結合制御因子の同定のためのシングル核RNAseq解析を再度実施し、前年度より腱細胞が明確にクラスター形成された結果を取得できた。今後は2022年度、2023年度の結果の解析から骨格筋の分化に関与する因子や筋腱相互作用因子の候補を選抜し、マウス胚における発現解析や培養細胞を用いた機能解析を進める。課題2腱骨境界で発現するnon-coding RNAの解析については、標的とするRNAのexon1を欠損させたノックアウトマウス系統の骨格の解析から一部の筋付着部の形態に異常が見出された。さらに同RNAのexon1-6を全て欠損したマウス系統も樹立できたため、今後これら2系統マウスを解析していくことで腱骨境界形成におけるこのnoncoding RNAの機能を解明していく。課題3Scx標的遺伝子の機能解析については標的遺伝子近傍配列のScxによる転写制御領域を絞り込むことができた。また、ノックアウトマウスの解析から腱組織中の腱細胞の形態や配置に変化がある可能性が見出された。今後はScxと制御配列の直接的な結合を確かめるとともに、ノックアウトマウスの解析を進め、当該遺伝子の腱形成や筋・骨との相互作用における役割を解明する。

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  • 腱を中心とした運動器形態形成メカニズムの解明

    研究課題/領域番号:22H02636  2022年4月 - 2025年3月

    日本学術振興会  科学研究費助成事業  基盤研究(B)

    乾 雅史

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    配分額:17680000円 ( 直接経費:13600000円 、 間接経費:4080000円 )

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  • ハプロ不全優性遺伝病発症・重篤化の根幹となるエピジェネティックなゆらぎ

    研究課題/領域番号:21H04755  2021年4月 - 2024年3月

    日本学術振興会  科学研究費助成事業  基盤研究(A)

    大鐘 潤, 乾 雅史, 長嶋 比呂志

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    配分額:42120000円 ( 直接経費:32400000円 、 間接経費:9720000円 )

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  • 由来の異なる筋肉と腱はいかにして出会うのか

    研究課題/領域番号:19K06697  2019年4月 - 2022年3月

    日本学術振興会  科学研究費助成事業  基盤研究(C)

    乾 雅史

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    配分額:4290000円 ( 直接経費:3300000円 、 間接経費:990000円 )

    本研究は脊椎動物ではほとんど明らかになっていない、腱から骨格筋への情報伝達による筋配向制御メカニズムを明らかにすることを目的とした。そのために、発生中の胚から腱を除去するアプローチで腱から骨格筋への情報伝達の重要性を示した。またその際に発現変動する遺伝子群から筋腱結合を制御する因子の同定を試みた。本研究の結果から、筋腱境界領域に発現し、結合形成に関与する可能性のある20以上の遺伝子群を同定し、またiGonad法を用いた遺伝子ノックダウンから筋腱結合を制御しうる分泌遺伝子ファミリーを1つ同定した。本研究の結果から、発生中の胚の筋腱相互作用について多数の新たな知見が見出された。

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  • ゲノム編集技術を利用したアレル特異的染色体切断によるトリソミックレスキュー誘導

    研究課題/領域番号:16K15242  2016年4月 - 2018年3月

    日本学術振興会  科学研究費助成事業  挑戦的萌芽研究

    原 万里, 脇田 幸子, 橋詰 令太郎, 一志 真子, 宮川 世志幸, 乾 雅史

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    配分額:3640000円 ( 直接経費:2800000円 、 間接経費:840000円 )

    ダウン症候群の人由来iPS細胞から、ゲノム編集技術を用いて任意の21番染色体1本を消去し、21番染色体の組み合わせの異なる誘導型disomy 21細胞を複数株樹立した。これら誘導型disomy 21細胞における、消去された21番染色体の特定がSTR解析によりなされ、結果、3本の21番染色体のうちの2本から構成される、3通りの組み合わせの細胞株に分類された。これらの細胞株の配列情報の比較から、最終的に3本の21番染色体を染色体全長にわたり区別するフェイジングに成功した。以上の解析情報から、21番染色体をアレル特異的に複数部位で切断するCRISPR/Cas9システムの構築に成功した。

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  • SOX9翻訳後修飾による骨格形成制御メカニズムの解析

    研究課題/領域番号:16K18558  2016年4月 - 2018年3月

    日本学術振興会  科学研究費助成事業  若手研究(B)

    乾 雅史

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    配分額:4290000円 ( 直接経費:3300000円 、 間接経費:990000円 )

    SOX9は軟骨分化のマスター転写因子であり、正確な骨格形成にはその活性が定量的に厳密に制御されている必要があることが示されているが、そのためのメカニズムは十分解明されていない。本研究ではSOX9タンパク質の翻訳後修飾に着目し、SUMO化の標的アミノ酸であるK396に点変異を導入したマウスを作製・解析を行った。その結果、SOX9K396Rマウスは低身長・低体重であり骨格に異常が見られたことから、正確な骨格の形成にはSOX9K396に対する翻訳後修飾が重要であることが示唆された。また、SUMO化SOX9は野生型SOX9に対して抑制的に働くことが示され、今後はその詳細なメカニズムの解明が期待される。

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  • Mkxを介した腱・靭帯の再生と維持機構の解明

    研究課題/領域番号:15H02560  2015年4月 - 2020年3月

    日本学術振興会  科学研究費助成事業  基盤研究(A)

    淺原 弘嗣, 森 雅樹, 乾 雅史

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    配分額:40950000円 ( 直接経費:31500000円 、 間接経費:9450000円 )

    本研究では、我々の同定した腱・靱帯に特異的な転写因子Mkxの腱・靱帯組織の発生と維持に必須の機能とそのメカニズムを解明し、Mkxを用いた幹細胞からの腱・靱帯再生研究を行った。本研究の遂行においては、疾患研究・医療応用を目標に、ヒト組織と組織幹細胞・iPS技術を用いた研究を行い、細胞ベースでのゲノムワイドな研究を有機的に組み合わせることで、Mkxを起点とした、腱・靱帯の分子ネットワークを解明した。また、Mkx遺伝子改変ラットの作成を行い、これを利用することで腱・靱帯の維持・再生シグナルを解明した。

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  • TGFβクロストーク制御因子の探索と解析

    研究課題/領域番号:25871177  2013年4月 - 2015年3月

    日本学術振興会  科学研究費助成事業  若手研究(B)

    乾 雅史

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    配分額:4420000円 ( 直接経費:3400000円 、 間接経費:1020000円 )

    本研究はTGFβシグナルと細胞内外のシグナルのクロストークに焦点を当て、ハイスループット・スクリーニングとシグナル依存性の検証を組み合わせることで新規のクロストークTGFβ制御因子を探索した。HEK293T細胞およびTGFβレポーターを用い約16000の遺伝子をスクリーンし、異なるシグナル依存性のTGFβシグナル制御因子が複数同定された。これらの因子は全て新規のTGFβシグナル制御因子であり、かつTGFβシグナルと他のシグナル伝達系とのクロストークの焦点となるため、今後制御の分子メカニズムや個体レベルにおける役割を解析することで新たなシグナルクロストークの意義が明らかになることが期待される。

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  • ツメガエルの細胞接着と受容体に関する分子生物学的研究

    研究課題/領域番号:03J11882  2003年 - 2005年

    日本学術振興会  科学研究費助成事業  特別研究員奨励費

    乾 雅史

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    配分額:2700000円 ( 直接経費:2700000円 )

    私はDNAマイクロアレイの手法を用いてアフリカツメガエルの循環器系組織において発現する新規遺伝子を探索した。
    Stage 12.5(後期原腸胚)、20(後期神経胚)、26(尾芽胚)のツメガエル胚を外科的に予定心臓血管領域とそれ以外に切り分け、それぞれからRNAを抽出してプローブを作成した。これらのプローブを我々の研究室でデザインされたXenopus 8kマイクロアレイにハイブリダイズさせて遺伝子の発現を比較した結果、予定心臓血管領域における発現量がそれ以外の領域よりも2倍以上高い遺伝子を172見出し、そのうち既知の配列との相同性の低い15遺伝子の部分配列を単離した。Whole-mount in situ hybridization(WISH)法によりそれらの遺伝子の発現領域を検討した結果、そのうち3遺伝子が発生過程の循環器系の組織で明らかな発現を示した。この3遺伝子の中の一つについて、私はその幼生期における発現パターンからAmiと命名し、詳細な発現パターンと発生における役割について解析した。Amiの予想アミノ酸配列はヒトComplement Factor D、マウスAdipsinと約47%及び42%の相同性を示したが、ツメガエル成体におけるAmi mRNQの発現にはこれら哺乳類ホモログの発現と異なる点が観察されたため、これらが相同遺伝子であるかを結論するには蛋白質機能の比較など更なる検証が必要である。発生過程のAmiのmRNAは神経胚の前方腹側及び沿軸領域、尾芽胚期の前方腹側領域に発現し、幼生期には形成過程の血管に沿った発現が観察された。この幼生期の血管に沿った発現はこれまでに知られているいずれのマーカー遺伝子よりも明瞭であり、この遺伝子の発現パターンから血管形成の前方から後方への経時的な進行や、腹側における左右非対称性を観察することができた。

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