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  2. 久米 晃啓

久米 晃啓

クメ アキヒロ  (Akihiro Kume)

基本情報

所属
自治医科大学 附属病院臨床研究センター企画開発部 教授
学位
博士(医学)(東北大学)
J-GLOBAL ID
200901072254016208
researchmap会員ID
1000193248

研究キーワード

 3

研究分野

 4

経歴

 9
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学歴

 2

委員歴

 2

論文

 124
  • Yuji Kashiwakura, Kazuhiro Endo, Atsushi Ugajin, Tomohiro Kikuchi, Shuji Hishikawa, Hitoyasu Nakamura, Yuko Katakai, Nemekhbayar Baatartsogt, Takafumi Hiramoto, Morisada Hayakawa, Nobuhiko Kamoshita, Shoji Yamazaki, Akihiro Kume, Harushi Mori, Naohiro Sata, Yoichi Sakata, Shin-ichi Muramatsu, Tsukasa Ohmori
    Molecular Therapy - Methods & Clinical Development 2023年8月  
  • 柏倉 裕志, 遠藤 和洋, 宇賀神 敦, 菊地 智博, 菱川 修司, 中村 仁康, 片貝 祐子, Nemekhbayar Baatartsogt, 平本 貴史, 早川 盛禎, 鴨下 信彦, 山崎 晶司, 久米 晃啓, 森 墾, 佐田 尚宏, 坂田 洋一, 村松 慎一, 大森 司
    日本血栓止血学会誌 34(2) 240-240 2023年5月  
  • Teruhide Yamaguchi, Eriko Uchida, Takashi Okada, Keiya Ozawa, Masafumi Onodera, Akihiro Kume, Takashi Shimada, Satoru Takahashi, Kenzaburo Tani, Yasutomo Nasu, Tomoji Mashimo, Hiroyuki Mizuguchi, Kohnosuke Mitani, Kazushige Maki
    Human gene therapy 31(19-20) 1043-1053 2020年10月  
    The development of genome-editing technology could lead to breakthrough gene therapy. Genome editing has made it possible to easily knock out or modify a target gene, while current gene therapy using a virus vector or plasmid hampering modification with respect to gene replacement therapies. Clinical development using these genome-editing tools is progressing rapidly. However, it is also becoming clear that there is a possibility of unintended gene sequence modification or deletion, or the insertion of undesired genes, or the selection of cells with abnormalities in the cancer suppressor gene p53; these unwanted actions are not possible with current gene therapy. The Science Board of the Pharmaceuticals and Medical Devices Agency of Japan has compiled a report on the expected aspects of such genome-editing technology and the risks associated with it. This article summarizes the history of that discussion and compares the key concepts with information provided by other regulatory authorities.
  • Miyata S, Tominaga K, Sakashita E, Urabe M, Onuki Y, Gomi A, Yamaguchi T, Mieno M, Mizukami H, Kume A, Ozawa K, Watanabe E, Kawai K, Endo H
    Scientific reports 9(1) 9787 2019年7月  査読有り
  • Fumio Kurosaki, Ryosuke Uchibori, Yoshihide Sehara, Yasushi Saga, Masashi Urabe, Hiroaki Mizukami, Koichi Hagiwara, Akihiro Kume
    Human gene therapy 29(11) 1242-1251 2018年11月  査読有り
    Idiopathic pulmonary fibrosis (IPF) is a fibroproliferative disorder with limited therapeutic options. An aberrant wound healing process in response to repetitive lung injury has been suggested for its pathogenesis, and a number of cytokines including transforming growth factor β1 play pivotal roles in the induction and progression of fibrosis. Thus, the regulation of these pro-inflammatory conditions may reduce the progression of IPF and ameliorate its symptoms in patients. Interleukin-10 (IL-10), a pleiotropic cytokine, exerts anti-inflammatory and anti-fibrotic effects in numerous biological settings. In the present study, we investigated the preventive effects of IL-10 on bleomycin-induced pulmonary fibrosis in mice with the continuous expression of this cytokine via an adeno-associated virus serotype 6 vector. Mice were administered the adeno-associated virus serotype 6 vector encoding mouse IL-10 by intratracheal injection, and osmotic minipumps containing bleomycin were subcutaneously implanted seven days later. Lung histology and the expression levels of pro-inflammatory cytokines and fibrogenic cytokines were then analyzed. In mice exhibiting persistent IL-10 expression on day 35, the number of infiltrated inflammatory cells and the development of fibrosis in lung tissues were significantly reduced. Increases in transforming growth factor β1 and decreases in IFN-γ were also suppressed in treated animals, with changes in these cytokines playing important roles in the pathogenesis of pulmonary fibrosis. Furthermore, IL-10 significantly improved survival in bleomycin-induced mice. Our results provide insights into the potential benefit of the anti-fibrotic effects of IL-10 as a novel therapeutic approach for IPF.
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MISC

 173
  • KM Matsuda, A Kume, R Xu, Y Ueda, M Urabe, M Hasegawa, K Ozawa
    BLOOD 92(10) 150A-150A 1998年11月  
  • KM Matsuda, Y Ueda, M Urabe, M Hasegawa, A Kume, K Ozawa
    CANCER GENE THERAPY 5(6) S14-S14 1998年11月  
  • K Kogure, M Urabe, A Kume, Y Sato, K Ozawa
    BLOOD 92(10) 378B-378B 1998年11月  
  • H Kodaira, A Kume, Y Ogasawara, M Urabe, K Kitano, A Kakizuka, K Ozawa
    JAPANESE JOURNAL OF CANCER RESEARCH 89(7) 741-747 1998年7月  
    Several cancer gene therapy strategies involve suicide genes to kill the neoplasm, or to regulate effector cells such as lymphocytes, We have developed an inducible apoptosis system with a Fas-estrogen receptor fusion protein (MfasER) for rapid elimination of transduced cells. In the present study, we further improved this molecular switch for estrogen-inducible apoptosis to overcome concerns with the wild-type estrogen receptor and its natural ligand, 17 beta-estradiol (E-2). The ligand-binding domain of MfasER was replaced with that of a mutant estrogen receptor which is unable to bind estrogen yet retains affinity for a synthetic ligand, 4-hydroxytamoxifen (Tm), The resultant fusion protein (MfasTmR) and MfasER were expressed in L929 cells for examination of their ligand specificities. Tm induced apoptosis in MfasTmR-expressing cells (L929MfasTmR) at 10(-8) M or higher concentrations, but induced no apoptosis in MfasER-expressing cells (L929MfasER) at up to 10(-6) M, On the other hand, E-2 induced apoptosis in L929MfasER at concentrations as low as 10(-10)-10(-9) M, while it did so partially in L929MfasTmR at concentrations greater than 10(-7) M, Thus, L929MfasTmR cells were highly susceptible to Tm, but refractory to E-2, with 100-1,000 times more tolerance than L929MfasER, These results suggest that the MfasTmR/Tm system would induce apoptosis in the target cells more safely in vitro, working independently of endogenous estrogen.
  • M Kokubun, A Kume, M Urabe, H Mano, M Okubo, R Kasukawa, A Kakizuka, K Ozawa
    GENE THERAPY 5(7) 923-929 1998年7月  
    We investigated the feasibility of an inducible apoptosis system to regulate cells genetically engineered for ectopic cytokine production. In a previous study, cDNA encoding the ligand-binding domain of the rate estrogen receptor was fused to the sequence for murine Fas transmembrane and cytoplasmic regions, and expression of the fusion protein (MfasER) in L929 fibroblasts resulted in estrogen-dependent apoptosis. We applied this MfasER/estrogen strategy to apoptosis-mediated regulation of cytokine production, using the human granulocyte colony-stimulating factor (G-CSF) as a model. Upon estrogen treatment, the G-CSF producers expressing MfasER showed an apoptotic phenotype and died in several hours, with termination of G-CSF production. This estrogen-induced apoptosis: was not influenced by whether the target cells were proliferating or resting, unlike a conventional suicide system involving the herpes simplex virus I thymidine kinase (HSVtk). That is, estrogen induced prompt and extensive apoptosis in the resting cells which expressed MfasER, while ganciclovir treatment induced only partial reduction of the resting cells which expressed HSVtk. These results imply the feasibility of apoptosis-mediated regulation of cytokine production by genetically modified cells for supplement gene therapy.
  • DS Fan, M Ogawa, K Ikeguchi, K Fujimoto, M Urabe, A Kume, M Nishizawa, N Matsushita, K Kiuchi, H Ichinose, T Nagatsu, GJ Kurtzman, Nakano, I, K Ozawa
    NEUROSCIENCE LETTERS 248(1) 61-64 1998年5月  
    Glial cell line-derived neurotrophic factor (GDNF) is known as a potent neurotrophic factor for dopaminergic neurons. Since adeno-associated virus (AAV) vector is a suitable vehicle for gene transfer into neurons, rat E14 mesencephalic cells were transduced with an AAV vector expressing GDNF. When compared with mock transduction, a larger number of dopaminergic neurons survived in AAV-GDNF-transduced cultures (234% and 325% of controls at 1 and 2 weeks, respectively; P < 0.01). Furthermore, the dopaminergic neurons in the latter cultures grew more prominent neurites than those in the former. These findings suggest that AAV vector-mediated GDNF gene transfer may prevent dopaminergic neuron death, and is therefore a logical approach for the treatment of Parkinson's disease. (C) 1998 Elsevier Science Ireland Ltd.
  • 金沢丈治, 卜部匡司, 久米晃啓, 小沢敬也, KURTZMAN G J, 西野宏, 喜多村健
    頭頚部腫よう 24(2) 199 1998年5月  
  • 久米 晃啓
    International journal of hematology 67(3) 10-10 1998年4月  
  • A Kume, Y Ueda, K Ito, K Matsuda, M Urabe, H Mano, K Ozawa
    BLOOD 90(10) 2474-2474 1997年11月  
  • A Kume, K Matsuda, Y Ueda, M Urabe, T Suda, K Ozawa
    BLOOD 90(10) 516-516 1997年11月  
  • A Kume, H Nishiura, J Suda, T Suda
    BLOOD 89(9) 3434-3442 1997年5月  
    The involvement of focal adhesion kinase (FAK) in myeloid differentiation was investigated in primary murine bone marrow (BM) cells, In unstimulated BM, FAK mRNA was defected in myeloid and lymphoid cells, but not in erythroid precursors. When the BM cells were incubated with granulo-cyte-macrophage colony-stimulating factor (GM-CSF) or interleukin-3 (IL-3), FAK expression showed a remarkable difference depending on the cytokine. Although FAK was upregulated in the cells stimulated by GM-CSF (GM-treated cells), the kinase was barely detectable in the cells cultured with IL-3 (IL-3-treated cells). Morphology and flow cytometry analysis showed GM-CSF promoted the growth and differentiation of monocyte/macrophage lineage stronger than IL-3. In addition, motility of the cytokine-differentiated cells showed an overt distinction between the cultures, which was closely correlated with FAK expression. After 7 days of stimulation, GM-treated cells showed active migration and chemoattractant-induced morphologic polarization. In contrast, IL-3-treated cells showed minimal migration and polarization. These results suggest an important role of GM-CSF in the terminal differentiation of monocytes/macrophages, and possible involvement of FAK in functional maturity of this lineage. (C) 1997 by The American Society of Hematology.
  • CJ Ding, A Kume, H Bjorgvinsdottir, RG Hawley, N Pech, MC Dinauer
    BLOOD 88(5) 1834-1840 1996年9月  
    The X-linked form of chronic granulomatous disease (X-CGD) results from mutations in the gene encoding gp91(phox), a 91-kD membrane glycoprotein that is the larger subunit of the respiratory burst oxidase cytochrome b. In this study, a new retroviral vector for expression of human gp91(phox), MSCV-h91Neo, based on murine stem cell virus vectors, was evaluated using a human X-CGD myeloid cell line (X-CGD PLB-985 cells) and murine bone marrow cells. Expression of recombinant gp91(phox) in transduced X-CGD PLB-985 cells was substantially improved compared with levels achieved previously using a different retroviral construct, and respiratory burst oxidase activity was fully reconstituted in the majority of clones analyzed. Expression of gp91(phox) transcripts was also observed in primary and secondary murine colony-forming unit-spleen derived from transduced bone marrow cells. Furthermore, respiratory burst activity was restored to granulocyte-monocyte progeny of transduced X-CGD mice bone marrow cells cultured in vitro. This observation is the first reported use of gene transfer to correct the enzymatic defect in murine CGD phagocytes and is also consistent with the high conservation of the oxidase complex among different species. Taken together, these data suggest that the MSCV-h91Neo vector may be useful for gene replacement therapy in X-linked CGD, in which high-level reconstitution of phagocyte oxidase activity may be important for full correction of phagocyte microbicidal function. (C) 1996 by The American Society of Hematology.
  • C Ding, N Pech, A Kume, MC Dinauer
    BLOOD 86(10) 956-956 1995年11月  
  • A KUME, MC DINAUER
    BLOOD 84(10) 3311-3316 1994年11月  
    X-linked chronic granulomatous disease (X-CGD) results from mutations in the gene encoding gp91(phox), the larger subunit of the respiratory burst oxidase cytochrome b. In this study, a recombinant retrovirus vector was constructed and evaluated for its expression of human gp91(phox) in a human X-CGD myeloid cell line in which the endogenous gp91(phox) gene had been disrupted by gene targeting. The retrovirus construct, Zip/PGKgp91, was first introduced into the GP+envAm12 amphotropic packaging line and yielded virus producer clones with estimated titers of up to 1 x 10(5) cfu/mL. Coculture infection of X-CGD myeloid cells with Zip/ PGKgp91 resulted in restoration of respiratory burst activity to 15% of the cells. Isolated clonal infectants expressed relatively low levels of recombinant gp91(phox) (less than or equal to 12% of wild-type), but exhibited considerable superoxide-generating activity (up to nearly 60% of wild-type). These results show the feasibility of phenotypic correction of CGD using gene replacement therapy and suggest that even modest levels of gp91(phox) expression may lead to considerable functional correction of X-CGD neutrophils. (C) 1994 by The American Society of Hematology.
  • A KUME, MC DINAUER
    BLOOD 82(10) A320-A320 1993年11月  
  • K TADA, S KURE, M TAKAYANAGI, A KUME, K NARISAWA
    EARLY HUMAN DEVELOPMENT 29(1-3) 75-81 1992年6月  
    Non-ketotic hyperglycinemia (NKH) is a well-recognized metabolic cause of life-threatening illness in the neonate. The fundamental defect is in the glycine cleavage enzyme (GCE), which consists of four protein components. Our study revealed that the majority of NKH patients had a specific defect in P-protein (glycine decarboxylase). The primary lesion of NKH in gene level was investigated, using cDNA encoding human glycine decarboxylase. A three-base deletion; resulting in deletion of Phe756 was found in a Japanese patient with NKH. In the majority of NKH patients in Finland, where there is a high incidence of NKH, it was found to be due to a common mutation - a point mutation resulting in amino acid alternation from Ser564 to Ile564. Prenatal diagnosis is possible by determining the activity of GCE and also by DNA analysis. Recent findings suggest that the high concentrations of glycine in the brain may contribute to the pathophysiology of NKH by overactivating NMDA receptors via an action at the associated glycine modulatory site. These provide a possibility that early treatment with NMDA receptor antagonist may prevent brain damage in NKH.
  • S KURE, H KOYATA, A KUME, Y ISHIGURO, K HIRAGA
    JOURNAL OF BIOLOGICAL CHEMISTRY 266(5) 3330-3334 1991年2月  
    Regulation of the transcription of the glycine decarboxylase gene and the H-protein gene was examined in chicken. Northern analysis suggested and run-off transcription confirmed that the glycine decarboxylase gene transcription is exclusively tissue-specific and takes place at different efficiencies in liver, kidney, and brain which are the chicken tissues exhibiting the glycine cleavage activity. No evidence for the glycine decarboxylase gene transcription was obtained in heart, spleen, and skeletal muscle. Basal and tissue-specific transcription of the H-protein gene can be distinguished. The tissue-specific transcription coordinates with transcription of the glycine decarboxylase gene in active tissues, while low abundance H-protein and its mRNA, products of the basal transcription, exist in inactive tissues with small amounts of T-protein. Apparently, T-protein is synthesized by a process similar to that for H-protein. Glycine decarboxylase mRNA levels show a linear relationship with H-protein mRNA levels and with specific activities of the glycine cleavage reaction in active tissues. Tissue-specific distribution of the glycine cleavage activity is primarily determined by the expression of the glycine decarboxylase gene. The coordinate and tissue-specific transcription of the genes for the constituent proteins plays a key role in determining the magnitude of the glycine cleavage activity in chicken tissues and, thereby, the tissue-specificity of glycine metabolism.
  • A KUME, H KOYATA, T SAKAKIBARA, Y ISHIGURO, S KURE, K HIRAGA
    JOURNAL OF BIOLOGICAL CHEMISTRY 266(5) 3323-3329 1991年2月  
    A cDNA encoding chicken glycine decarboxylase (pCP15b) was isolated using an antibody specific to this protein. Additional cDNAs were cloned with the aid of the genomic fragments obtained by using the pCP15b cDNA probe. No initiator methionine codon is found in the currently elucidated cDNA sequence, and an ATG codon in an exon is assigned to this role. The precursor glycine decarboxylase deduced from the 3514-base pair nucleotide sequence is comprised of 1,004 amino acids (M(r) = 111,848). The 1,020 amino acid residues are encoded for the precursor form of human glycine decarboxylase (M(r) = 112,869) in the 3,783-base long cDNA sequence of two 1.9-kilobase pair cDNAs with a pentanucleotide overlap. The pyridoxal phosphate binding site lysine and a glycine-rich region, which is suggested to be responsible for the attachment of the phosphate moiety of pyridoxal phosphate, are found in close proximity in both the chicken and human enzymes. This region essential for the enzyme action is suggested to be embedded in a segment rich in beta-turns and random coils and is surrounded by conserved and repetitive amino acid sequences. It is suggested that these structures are involved in the organization of the active site of glycine decarboxylase.
  • Journal of Inherited Metabolic Disease 13(5) 766 1991年  
  • T SAKAKIBARA, H KOYATA, Y ISHIGURO, S KURE, A KUME, K TADA, K HIRAGA
    BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS 173(3) 801-806 1990年12月  
  • 多田 啓也, 久米 晃啓, 呉 繁夫
    厚生省神経疾患研究委託費研究報告書 代謝障害に基づく中枢神経疾患の発症機構と治療に関する研究 平成元年度 14-17 1990年3月  
    P蛋白欠損の遺伝子レベルの異常を明らかにする目的で,P蛋白をコードするcDNAのクローニングを行い,このcDNAをプローブとして本症症例の遺伝子解析を行った.8例の非ケトーシス型高グリシン血症の中1例に於てSouthern法により遺伝子の部分欠失が認められた.他の7例は本法では検出可能な異常は見出されず,恐らく点変異に基づくものと推定された
  • A KUME, S KURE, K TADA, K HIRAGA
    BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS 154(1) 292-297 1988年7月  
  • Stem Cells 17(4) 226-232  

書籍等出版物

 1

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 8
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 2

共同研究・競争的資金等の研究課題

 27
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