=== Generating (published_papers) === === Generating (research_interests) === === Generating (teaching_experience) === === Generating (misc) === === Generating (research_projects) === === Generating (books_etc) === === Generating (awards) === === Generating (association_memberships) === === Generating (presentations) === ==== begin registerFile(/WWW/pub2/data/ERD/person/246724/researchmap/published_papers.jsonl) ==== line:1, {"insert":{"user_id":"R000014847","type":"published_papers","id":"41379213"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/36761774","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=400453","label":"url"}],"paper_title":{"en":"Negative interference with antibody-dependent cellular cytotoxicity mediated by rituximab from its interactions with human serum proteins","ja":"Negative interference with antibody-dependent cellular cytotoxicity mediated by rituximab from its interactions with human serum proteins"},"authors":{"en":[{"name":"Yanaka Saeko"},{"name":"Yogo Rina"},{"name":"Yagi Hirokazu"},{"name":"Onitsuka Masayoshi"},{"name":"Wakaizumi Natsumi"},{"name":"Yamaguchi Yuki"},{"name":"Uchiyama Susumu"},{"name":"Kato Koichi"}],"ja":[{"name":"Yanaka Saeko"},{"name":"Yogo Rina"},{"name":"Yagi Hirokazu"},{"name":"鬼塚 正義"},{"name":"Wakaizumi Natsumi"},{"name":"Yamaguchi Yuki"},{"name":"Uchiyama Susumu"},{"name":"Kato Koichi"}]},"description":{"en":"Although interactions of small molecular drugs with serum proteins have been widely studied from pharmacokinetic and pharmacodynamic perspectives, there have been few reports on the effects of serum components on therapeutic antibody functions. This study reports the effect of abundant serum proteins on antibody-dependent cellular cytotoxicity (ADCC) mediated by rituximab and Fcγ receptor III (FcγRIII). Human serum albumin (HSA) and the Fab fragment from the pooled serum polyclonal IgG were found to compromise ADCC as non-competitive inhibitors. Our nuclear magnetic resonance data provided direct evidence for the interactions of HSA with both the Fab and Fc regions of rituximab and also with the extracellular region of FcγRIII (sFcγRIII). The degree of involvement in the interaction decreased in the order of rituximab-Fab > rituximab-Fc > sFcγRIII, suggesting preferential binding of HSA to net positively charged proteins. Although much less pronounced than the effect of HSA, polyclonal IgG-Fab specifically interacted with rituximab-Fc. The NMR data also showed that the serum protein interactions cover the Fc surface extensively, suggesting that they can act as pan-inhibitors against various Fc receptor-mediated functions and pharmacokinetics. Our findings highlight the importance of considering serum-protein interactions in the design and application of antibody-based drugs with increased efficacy and safety.","ja":"Although interactions of small molecular drugs with serum proteins have been widely studied from pharmacokinetic and pharmacodynamic perspectives, there have been few reports on the effects of serum components on therapeutic antibody functions. This study reports the effect of abundant serum proteins on antibody-dependent cellular cytotoxicity (ADCC) mediated by rituximab and Fcγ receptor III (FcγRIII). Human serum albumin (HSA) and the Fab fragment from the pooled serum polyclonal IgG were found to compromise ADCC as non-competitive inhibitors. Our nuclear magnetic resonance data provided direct evidence for the interactions of HSA with both the Fab and Fc regions of rituximab and also with the extracellular region of FcγRIII (sFcγRIII). The degree of involvement in the interaction decreased in the order of rituximab-Fab > rituximab-Fc > sFcγRIII, suggesting preferential binding of HSA to net positively charged proteins. Although much less pronounced than the effect of HSA, polyclonal IgG-Fab specifically interacted with rituximab-Fc. The NMR data also showed that the serum protein interactions cover the Fc surface extensively, suggesting that they can act as pan-inhibitors against various Fc receptor-mediated functions and pharmacokinetics. Our findings highlight the importance of considering serum-protein interactions in the design and application of antibody-based drugs with increased efficacy and safety."},"publication_date":"2023-01-25","publication_name":{"en":"Frontiers in Immunology","ja":"Frontiers in Immunology"},"volume":"Vol.14","languages":["eng"],"referee":true,"identifiers":{"doi":["10.3389/fimmu.2023.1090898"],"issn":["1664-3224"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:2, {"insert":{"user_id":"R000014847","type":"published_papers","id":"37030825"},"force":{"see_also":[{"@id":"https://repo.lib.tokushima-u.ac.jp/ja/117739","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=385877","label":"url"}],"paper_title":{"en":"Reversal of neuroinflammation in novel galactosialidosis model mice by single intracerebroventricular administration of CHO-derived human recombinant cathepsin A precursor protein.","ja":"Reversal of neuroinflammation in novel galactosialidosis model mice by single intracerebroventricular administration of CHO-derived human recombinant cathepsin A precursor protein."},"authors":{"en":[{"name":"Horii Yuto"},{"name":"Iniwa Toshiki"},{"name":"Onitsuka Masayoshi"},{"name":"Tsukimoto Jun"},{"name":"Tanaka Yuki"},{"name":"Ike Hironobu"},{"name":"Fukushi Yuri"},{"name":"Andoh Haruna"},{"name":"Takeuchi Yoshie"},{"name":"Nishioka So-ichiro"},{"name":"Tsuji Daisuke"},{"name":"Ikuo Mariko"},{"name":"Yamazaki Naoshi"},{"name":"Takiguchi Yoshiharu"},{"name":"Ishimaru Naozumi"},{"name":"Itou Kouji"}],"ja":[{"name":"堀井 雄登"},{"name":"五百磐 俊樹"},{"name":"鬼塚 正義"},{"name":"月本 準"},{"name":"Tanaka Yuki"},{"name":"池 啓伸"},{"name":"福士 友理"},{"name":"安藤 春菜"},{"name":"竹内 美絵"},{"name":"西岡 宗一郎"},{"name":"辻 大輔"},{"name":"幾尾 真理子"},{"name":"山﨑 尚志"},{"name":"滝口 祥令"},{"name":"石丸 直澄"},{"name":"伊藤 孝司"}]},"publication_date":"2022-06-15","publication_name":{"en":"Molecular Therapy. Methods & Clinical Development","ja":"Molecular Therapy. Methods & Clinical Development"},"volume":"Vol.25","number":"No.June","starting_page":"297","ending_page":"310","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.omtm.2022.04.001"],"issn":["2329-0501"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:3, {"insert":{"user_id":"R000014847","type":"published_papers"},"similar_merge":{"see_also":[{"@id":"https://repo.lib.tokushima-u.ac.jp/ja/117434","label":"url"},{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/34739851","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=390159","label":"url"}],"paper_title":{"en":"Live-cell imaging to analyze intracellular aggregation of recombinant IgG in CHO cells.","ja":"Live-cell imaging to analyze intracellular aggregation of recombinant IgG in CHO cells."},"authors":{"en":[{"name":"Senga Yukako"},{"name":"Doi Motomichi"},{"name":"Onitsuka Masayoshi"},{"name":"Honda Shinya"}],"ja":[{"name":"Senga Yukako"},{"name":"Doi Motomichi"},{"name":"鬼塚 正義"},{"name":"Honda Shinya"}]},"description":{"en":"Recombinant immunoglobulin G (IgG) aggregates are formed during their production. However, the process underlying intracellular/extracellular aggregation in cell culture conditions is not well understood, and no effective method exists to assess IgG aggregates. Here, we establish an approach to detect intracellular aggregates using AF.2A1, a small artificial protein that binds to non-native IgG conformers and aggregates. Fluorescent-labeled AF.2A1 is prepared via conjugation and transfected into antibody-producing Chinese hamster ovary (CHO) cells. Micrographic images show intracellular IgG aggregates in CHO cells. The relative amount of intracellular aggregates (versus total intracellular IgG) differed depending on the type of additives used during cell culture. Interestingly, the relative amount of intracellular aggregates moderately correlates with that of in vitro extracellular IgG aggregates, suggesting they are secreted. This method will allow the investigation of antibody aggregation in cells, and may guide the production of therapeutic antibodies with high yield/quality.","ja":"Recombinant immunoglobulin G (IgG) aggregates are formed during their production. However, the process underlying intracellular/extracellular aggregation in cell culture conditions is not well understood, and no effective method exists to assess IgG aggregates. Here, we establish an approach to detect intracellular aggregates using AF.2A1, a small artificial protein that binds to non-native IgG conformers and aggregates. Fluorescent-labeled AF.2A1 is prepared via conjugation and transfected into antibody-producing Chinese hamster ovary (CHO) cells. Micrographic images show intracellular IgG aggregates in CHO cells. The relative amount of intracellular aggregates (versus total intracellular IgG) differed depending on the type of additives used during cell culture. Interestingly, the relative amount of intracellular aggregates moderately correlates with that of in vitro extracellular IgG aggregates, suggesting they are secreted. This method will allow the investigation of antibody aggregation in cells, and may guide the production of therapeutic antibodies with high yield/quality."},"publication_date":"2022-01-20","publication_name":{"en":"Cell Chemical Biology","ja":"Cell Chemical Biology"},"volume":"Vol.29","number":"No.1","starting_page":"120","ending_page":"132","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.chembiol.2021.08.010"],"issn":["2451-9448"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:4, {"insert":{"user_id":"R000014847","type":"published_papers"},"similar_merge":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/34978013","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=390175","label":"url"}],"paper_title":{"en":"Glutamine-free mammalian expression of recombinant glycoproteins with uniform isotope labeling: an application for NMR analysis of pharmaceutically relevant Fc glycoforms of human immunoglobulin G1","ja":"Glutamine-free mammalian expression of recombinant glycoproteins with uniform isotope labeling: an application for NMR analysis of pharmaceutically relevant Fc glycoforms of human immunoglobulin G1"},"authors":{"en":[{"name":"Yanaka Saeko"},{"name":"Yagi Hirokazu"},{"name":"Yogo Rina"},{"name":"Onitsuka Masayoshi"},{"name":"Kato Koichi"}],"ja":[{"name":"Yanaka Saeko"},{"name":"Yagi Hirokazu"},{"name":"Yogo Rina"},{"name":"鬼塚 正義"},{"name":"Kato Koichi"}]},"description":{"en":"Mammalian cells are widely used for producing recombinant glycoproteins of pharmaceutical interest. However, a major drawback of using mammalian cells is the high production costs associated with uniformly isotope-labeled glycoproteins due to the large quantity of labeled L-glutamine required for their growth. To address this problem, we developed a cost-saving method for uniform isotope labeling by cultivating the mammalian cells under glutamine-free conditions, which was achieved by co-expression of glutamine synthase. We demonstrate the utility of this approach using fucosylated and non-fucosylated Fc glycoforms of human immunoglobulin G1.","ja":"Mammalian cells are widely used for producing recombinant glycoproteins of pharmaceutical interest. However, a major drawback of using mammalian cells is the high production costs associated with uniformly isotope-labeled glycoproteins due to the large quantity of labeled L-glutamine required for their growth. To address this problem, we developed a cost-saving method for uniform isotope labeling by cultivating the mammalian cells under glutamine-free conditions, which was achieved by co-expression of glutamine synthase. We demonstrate the utility of this approach using fucosylated and non-fucosylated Fc glycoforms of human immunoglobulin G1."},"publication_date":"2022-01-03","publication_name":{"en":"Journal of Biomolecular NMR","ja":"Journal of Biomolecular NMR"},"volume":"Vol.76","number":"No.1-2","starting_page":"17","ending_page":"22","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1007/s10858-021-00387-5"],"issn":["1573-5001"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:5, {"insert":{"user_id":"R000014847","type":"published_papers","id":"33247647"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/34119424","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=377856","label":"url"}],"paper_title":{"en":"Production of monoclonal shark-derived immunoglobulin new antigen receptor antibodies using Chinese hamster ovary cell expression system","ja":"Production of monoclonal shark-derived immunoglobulin new antigen receptor antibodies using Chinese hamster ovary cell expression system"},"authors":{"en":[{"name":"Enatsu Hajime"},{"name":"Okamoto Nako"},{"name":"Nomura Yoshiki"},{"name":"Onitsuka Masayoshi"},{"name":"Yamano-Adachi Noriko"},{"name":"Koga Yuichi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"Enatsu Hajime"},{"name":"Okamoto Nako"},{"name":"Nomura Yoshiki"},{"name":"鬼塚 正義"},{"name":"Yamano-Adachi Noriko"},{"name":"Koga Yuichi"},{"name":"大政 健史"}]},"description":{"en":"Cartilaginous fishes such as sharks have adaptive immune systems based on immunoglobulins similar to those in mammals. During their evolution, cartilaginous fishes individually have acquired their adaptive immune system called immunoglobulin new antigen receptor (IgNARs). IgNARs maintain their functions in the harsh environment of shark serum, which contains a high concentration of urea to prevent water loss in seawater. Therefore, IgNARs have high structural stability, and are expected to be used as next-generation antibodies in applications different from those of conventional IgG antibodies. However, no recombinant expression system for IgNAR, which has a molecular weight of approximately 147 kDa as a dimer and multiple N-glycosylation sites, has yet been constructed. This has stalled research into IgNAR development. Here, we constructed a recombinant expression system for IgNAR using Chinese hamster ovary (CHO) cells, widely used as hosts for IgG antibody production. Using this system, IgNAR was successfully expressed and purified as a human IgG Fc fusion protein and showed antigen-binding ability. After Protein A affinity purification, followed by specific cleavage and removal of the human Fc-region, the final yield of IgNAR was 1.07 mg/L-medium. Moreover, this CHO cell expression system modified IgNAR with various N-glycans, including high-mannose and complex types. This expression system will allow us to analyze the structure, physicochemical properties, and biological functions of IgNAR. This fundamental information will advance the development of IgNARs for industrial and biotechnological applications.","ja":"Cartilaginous fishes such as sharks have adaptive immune systems based on immunoglobulins similar to those in mammals. During their evolution, cartilaginous fishes individually have acquired their adaptive immune system called immunoglobulin new antigen receptor (IgNARs). IgNARs maintain their functions in the harsh environment of shark serum, which contains a high concentration of urea to prevent water loss in seawater. Therefore, IgNARs have high structural stability, and are expected to be used as next-generation antibodies in applications different from those of conventional IgG antibodies. However, no recombinant expression system for IgNAR, which has a molecular weight of approximately 147 kDa as a dimer and multiple N-glycosylation sites, has yet been constructed. This has stalled research into IgNAR development. Here, we constructed a recombinant expression system for IgNAR using Chinese hamster ovary (CHO) cells, widely used as hosts for IgG antibody production. Using this system, IgNAR was successfully expressed and purified as a human IgG Fc fusion protein and showed antigen-binding ability. After Protein A affinity purification, followed by specific cleavage and removal of the human Fc-region, the final yield of IgNAR was 1.07 mg/L-medium. Moreover, this CHO cell expression system modified IgNAR with various N-glycans, including high-mannose and complex types. This expression system will allow us to analyze the structure, physicochemical properties, and biological functions of IgNAR. This fundamental information will advance the development of IgNARs for industrial and biotechnological applications."},"publication_date":"2021-06-09","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"volume":"Vol.132","number":"No.3","starting_page":"302","ending_page":"309","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2021.04.015"],"issn":["1347-4421"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:6, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31426351"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/32878739","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-85090018528&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=373148","label":"url"}],"paper_title":{"en":"Effect of the disulfide isomerase PDIa4 on the antibody production of Chinese hamster ovary cells.","ja":"Effect of the disulfide isomerase PDIa4 on the antibody production of Chinese hamster ovary cells."},"authors":{"en":[{"name":"Komatsu Kei"},{"name":"Kumon Kento"},{"name":"Arita Mayuno"},{"name":"Onitsuka Masayoshi"},{"name":"Omasa Takeshi"},{"name":"Yohda Masafumi"}],"ja":[{"name":"Komatsu Kei"},{"name":"Kumon Kento"},{"name":"Arita Mayuno"},{"name":"鬼塚 正義"},{"name":"大政 健史"},{"name":"Yohda Masafumi"}]},"description":{"en":"Therapeutic monoclonal antibodies recognize and bind specific molecules on the surface of target cells, stimulating the immune system, which can attack these targeted cells. These antibodies are produced by mammalian cells, including Chinese hamster ovary (CHO) cells, because the formation of antibodies requires complicated posttranslational modifications, including peptidyl-prolyl cis/trans isomerization, disulfide bond formation, and glycosylation. Currently, it is thought that the efficient production of secretory proteins is limited by posttranslational processes. The ER is the biosynthesis site of all secreted and membrane proteins. The accumulation of unfolded proteins in the ER causes the ER stress response. During the ER stress state, various molecular chaperones are expressed to prevent proteins from the aggregate formation. The molecular chaperone involved in ER stress likely plays an essential role in the production of secretory proteins. The purpose of this study was to improve the production of monoclonal antibodies by cells. We elucidated the function of ER chaperones in the production of a monoclonal antibody. First, we quantitatively measured the mRNA expression levels of protein disulfide-isomerase family members. In CHO HcD6 cells treated with tunicamycin, the expression level of pdia4 was significantly increased. Second, we investigated the relationship between PDIa4 and antibody productivity in pdia4-knockdown cells. Both a decrease in the amount of secreted antibody and the accumulation of immature antibodies inside the cells were observed. Recombinant PDIa4 was able to refold the antibodies and Fabs. These results indicate that PDIa4 affects the production of monoclonal antibodies by catalyzing disulfide bond formation in these antibodies in CHO cells.","ja":"Therapeutic monoclonal antibodies recognize and bind specific molecules on the surface of target cells, stimulating the immune system, which can attack these targeted cells. These antibodies are produced by mammalian cells, including Chinese hamster ovary (CHO) cells, because the formation of antibodies requires complicated posttranslational modifications, including peptidyl-prolyl cis/trans isomerization, disulfide bond formation, and glycosylation. Currently, it is thought that the efficient production of secretory proteins is limited by posttranslational processes. The ER is the biosynthesis site of all secreted and membrane proteins. The accumulation of unfolded proteins in the ER causes the ER stress response. During the ER stress state, various molecular chaperones are expressed to prevent proteins from the aggregate formation. The molecular chaperone involved in ER stress likely plays an essential role in the production of secretory proteins. The purpose of this study was to improve the production of monoclonal antibodies by cells. We elucidated the function of ER chaperones in the production of a monoclonal antibody. First, we quantitatively measured the mRNA expression levels of protein disulfide-isomerase family members. In CHO HcD6 cells treated with tunicamycin, the expression level of pdia4 was significantly increased. Second, we investigated the relationship between PDIa4 and antibody productivity in pdia4-knockdown cells. Both a decrease in the amount of secreted antibody and the accumulation of immature antibodies inside the cells were observed. Recombinant PDIa4 was able to refold the antibodies and Fabs. These results indicate that PDIa4 affects the production of monoclonal antibodies by catalyzing disulfide bond formation in these antibodies in CHO cells."},"publication_date":"2020-12","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"volume":"Vol.130","number":"No.6","starting_page":"637","ending_page":"643","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2020.08.001"],"issn":["1347-4421"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:7, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31426352"},"force":{"see_also":[{"@id":"https://repo.lib.tokushima-u.ac.jp/ja/115880","label":"url"},{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/33114581","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-85094185161&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=373149","label":"url"}],"paper_title":{"en":"Silkworm pupae function as efficient producers of recombinant glycoproteins with stable-isotope labeling.","ja":"Silkworm pupae function as efficient producers of recombinant glycoproteins with stable-isotope labeling."},"authors":{"en":[{"name":"Yagi Hirokazu"},{"name":"Yanaka Saeko"},{"name":"Yogo Rina"},{"name":"Ikeda Akari"},{"name":"Onitsuka Masayoshi"},{"name":"Yamazaki Toshio"},{"name":"Kato Ttsuya"},{"name":"Park Y. Enoch"},{"name":"Yokoyama Jun"},{"name":"Kato Koichi"}],"ja":[{"name":"Yagi Hirokazu"},{"name":"Yanaka Saeko"},{"name":"Yogo Rina"},{"name":"Ikeda Akari"},{"name":"鬼塚 正義"},{"name":"Yamazaki Toshio"},{"name":"Kato Ttsuya"},{"name":"Park Y. Enoch"},{"name":"Yokoyama Jun"},{"name":"Kato Koichi"}]},"description":{"en":"Baculovirus-infected silkworms are promising bioreactors for producing recombinant glycoproteins, including antibodies. Previously, we developed a method for isotope labeling of glycoproteins for nuclear magnetic resonance (NMR) studies using silkworm larvae reared on an artificial diet containing N-labeled yeast crude protein extract. Here, we further develop this method by introducing a technique for the expression of isotope-labeled glycoproteins by silkworm pupae, which has several potential advantages relative to larvae-based techniques in terms of production yield, ease of handling, and storage. Here, we fed fifth instar larvae an artificial diet with an optimized composition containing [methyl-C]methionine, leading to pupation. Nine-day-old pupae were then injected with recombinant nucleopolyhedrovirus (BmNPV) bacmid for expression of recombinant human immunoglobulin G (IgG). From the whole-body homogenates of pupae, 0.35 mg/pupa of IgG was harvested, which is a yield that is five times higher than can be obtained from larvae. Recombinant IgG, thus prepared, exhibited mainly three kinds of pauci-mannose-type oligosaccharides and had a C-enrichment ratio of approximately 80%. This enabled selective observation of NMR signals originating from the methionyl methyl group of IgG, confirming its conformational integrity. These data demonstrate the utility of silkworm pupae as factories for producing recombinant glycoproteins with amino-acid-selective isotope labeling.","ja":"Baculovirus-infected silkworms are promising bioreactors for producing recombinant glycoproteins, including antibodies. Previously, we developed a method for isotope labeling of glycoproteins for nuclear magnetic resonance (NMR) studies using silkworm larvae reared on an artificial diet containing N-labeled yeast crude protein extract. Here, we further develop this method by introducing a technique for the expression of isotope-labeled glycoproteins by silkworm pupae, which has several potential advantages relative to larvae-based techniques in terms of production yield, ease of handling, and storage. Here, we fed fifth instar larvae an artificial diet with an optimized composition containing [methyl-C]methionine, leading to pupation. Nine-day-old pupae were then injected with recombinant nucleopolyhedrovirus (BmNPV) bacmid for expression of recombinant human immunoglobulin G (IgG). From the whole-body homogenates of pupae, 0.35 mg/pupa of IgG was harvested, which is a yield that is five times higher than can be obtained from larvae. Recombinant IgG, thus prepared, exhibited mainly three kinds of pauci-mannose-type oligosaccharides and had a C-enrichment ratio of approximately 80%. This enabled selective observation of NMR signals originating from the methionyl methyl group of IgG, confirming its conformational integrity. These data demonstrate the utility of silkworm pupae as factories for producing recombinant glycoproteins with amino-acid-selective isotope labeling."},"publication_date":"2020-10-26","publication_name":{"en":"Biomolecules","ja":"Biomolecules"},"volume":"Vol.10","number":"No.11","starting_page":"1482","ending_page":"1482","languages":["eng"],"referee":true,"identifiers":{"doi":["10.3390/biom10111482"],"issn":["2218-273X"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:8, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31426353"},"force":{"see_also":[{"@id":"https://repo.lib.tokushima-u.ac.jp/ja/115833","label":"url"},{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/32188928","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-85082085940&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=373147","label":"url"}],"paper_title":{"en":"Build-up functionalization of anti-EGFR × anti-CD3 bispecific diabodies by integrating high-affinity mutants and functional molecular formats.","ja":"Build-up functionalization of anti-EGFR × anti-CD3 bispecific diabodies by integrating high-affinity mutants and functional molecular formats."},"authors":{"en":[{"name":"Asano Ryutaro"},{"name":"Hosokawa Katsuhiro"},{"name":"Taki Shintaro"},{"name":"Konno Shota"},{"name":"Shimomura Ippei"},{"name":"Ogata Hiromi"},{"name":"Okada Mai"},{"name":"Arai Kyoko"},{"name":"Onitsuka Masayoshi"},{"name":"Omasa Takeshi"},{"name":"Nakanishi Takeshi"},{"name":"Umetsu Mitsuo"},{"name":"Kumagai Izumi"}],"ja":[{"name":"Asano Ryutaro"},{"name":"Hosokawa Katsuhiro"},{"name":"Taki Shintaro"},{"name":"Konno Shota"},{"name":"Shimomura Ippei"},{"name":"Ogata Hiromi"},{"name":"Okada Mai"},{"name":"Arai Kyoko"},{"name":"鬼塚 正義"},{"name":"大政 健史"},{"name":"Nakanishi Takeshi"},{"name":"Umetsu Mitsuo"},{"name":"Kumagai Izumi"}]},"description":{"en":"Designing non-natural antibody formats is a practical method for developing highly functional next-generation antibody drugs, particularly for improving the therapeutic efficacy of cancer treatments. One approach is constructing bispecific antibodies (bsAbs). We previously reported a functional humanized bispecific diabody (bsDb) that targeted epidermal growth factor receptor and CD3 (hEx3-Db). We enhanced its cytotoxicity by constructing an Fc fusion protein and rearranging order of the V domain. In this study, we created an additional functional bsAb, by integrating the molecular formats of bsAb and high-affinity mutants previously isolated by phage display in the form of Fv. Introducing the high-affinity mutations into bsDbs successfully increased their affinities and enhanced their cytotoxicity in vitro and in vivo. However, there were some limitations to affinity maturation of bsDb by integrating high-affinity Fv mutants, particularly in Fc-fused bsDb with intrinsic high affinity, because of their bivalency. The tetramers fractionated from the bsDb mutant exhibited the highest in vitro growth inhibition among the small bsAbs and was comparable to the in vivo anti-tumor effects of Fc-fused bsDbs. This molecule shows cost-efficient bacterial production and high therapeutic potential.","ja":"Designing non-natural antibody formats is a practical method for developing highly functional next-generation antibody drugs, particularly for improving the therapeutic efficacy of cancer treatments. One approach is constructing bispecific antibodies (bsAbs). We previously reported a functional humanized bispecific diabody (bsDb) that targeted epidermal growth factor receptor and CD3 (hEx3-Db). We enhanced its cytotoxicity by constructing an Fc fusion protein and rearranging order of the V domain. In this study, we created an additional functional bsAb, by integrating the molecular formats of bsAb and high-affinity mutants previously isolated by phage display in the form of Fv. Introducing the high-affinity mutations into bsDbs successfully increased their affinities and enhanced their cytotoxicity in vitro and in vivo. However, there were some limitations to affinity maturation of bsDb by integrating high-affinity Fv mutants, particularly in Fc-fused bsDb with intrinsic high affinity, because of their bivalency. The tetramers fractionated from the bsDb mutant exhibited the highest in vitro growth inhibition among the small bsAbs and was comparable to the in vivo anti-tumor effects of Fc-fused bsDbs. This molecule shows cost-efficient bacterial production and high therapeutic potential."},"publication_date":"2020-04","publication_name":{"en":"Scientific Reports","ja":"Scientific Reports"},"volume":"Vol.10","starting_page":"4913","ending_page":"4913","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1038/s41598-020-61840-3"],"issn":["2045-2322"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:9, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219002"},"force":{"see_also":[{"@id":"https://repo.lib.tokushima-u.ac.jp/ja/114953","label":"url"},{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/31420591","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=356929","label":"url"}],"paper_title":{"en":"The Fab portion of immunoglobulin G contributes to its binding to Fcγ receptor III","ja":"The Fab portion of immunoglobulin G contributes to its binding to Fcγ receptor III"},"authors":{"en":[{"name":"Yogo Rina"},{"name":"Yamaguchi Yuki"},{"name":"Watanabe Hiroki"},{"name":"Yagi Hirokazu"},{"name":"Satoh Tadashi"},{"name":"Nakanishi Mahito"},{"name":"Onitsuka Masayoshi"},{"name":"Omasa Takeshi"},{"name":"Shimada Mari"},{"name":"Maruno Takahiro"},{"name":"Torisu Tetsuo"},{"name":"Watanabe Shio"},{"name":"Higo Daisuke"},{"name":"Uchihashi Takayuki"},{"name":"Yanaka Saeko"},{"name":"Uchiyama Susumu"},{"name":"Kato Koichi"}],"ja":[{"name":"Yogo Rina"},{"name":"Yamaguchi Yuki"},{"name":"Watanabe Hiroki"},{"name":"Yagi Hirokazu"},{"name":"Satoh Tadashi"},{"name":"Nakanishi Mahito"},{"name":"鬼塚 正義"},{"name":"大政 健史"},{"name":"Shimada Mari"},{"name":"Maruno Takahiro"},{"name":"Torisu Tetsuo"},{"name":"Watanabe Shio"},{"name":"Higo Daisuke"},{"name":"Uchihashi Takayuki"},{"name":"Yanaka Saeko"},{"name":"Uchiyama Susumu"},{"name":"Kato Koichi"}]},"description":{"en":"Most cells active in the immune system express receptors for antibodies which mediate a variety of defensive mechanisms. These receptors interact with the Fc portion of the antibody and are therefore collectively called Fc receptors. Here, using high-speed atomic force microscopy, we observe interactions of human, humanized, and mouse/human-chimeric immunoglobulin G1 (IgG1) antibodies and their cognate Fc receptor, FcγRIIIa. Our results demonstrate that not only Fc but also Fab positively contributes to the interaction with the receptor. Furthermore, hydrogen/deuterium exchange mass spectrometric analysis reveals that the Fab portion of IgG1 is directly involved in its interaction with FcγRIIIa, in addition to the canonical Fc-mediated interaction. By targeting the previously unidentified receptor-interaction sites in IgG-Fab, our findings could inspire therapeutic antibody engineering.","ja":"Most cells active in the immune system express receptors for antibodies which mediate a variety of defensive mechanisms. These receptors interact with the Fc portion of the antibody and are therefore collectively called Fc receptors. Here, using high-speed atomic force microscopy, we observe interactions of human, humanized, and mouse/human-chimeric immunoglobulin G1 (IgG1) antibodies and their cognate Fc receptor, FcγRIIIa. Our results demonstrate that not only Fc but also Fab positively contributes to the interaction with the receptor. Furthermore, hydrogen/deuterium exchange mass spectrometric analysis reveals that the Fab portion of IgG1 is directly involved in its interaction with FcγRIIIa, in addition to the canonical Fc-mediated interaction. By targeting the previously unidentified receptor-interaction sites in IgG-Fab, our findings could inspire therapeutic antibody engineering."},"publication_date":"2019-08-16","publication_name":{"en":"Scientific Reports","ja":"Scientific Reports"},"volume":"Vol.9","number":"No.1","starting_page":"11957","ending_page":"11957","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1038/s41598-019-48323-w"],"issn":["2045-2322"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:10, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219003"},"force":{"see_also":[{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=356919","label":"url"}],"paper_title":{"en":"Characterization of Chinese hamster ovary cells with disparate chromosome numbers: Reduction of the amount of mRNA relative to total protein","ja":"Characterization of Chinese hamster ovary cells with disparate chromosome numbers: Reduction of the amount of mRNA relative to total protein"},"authors":{"en":[{"name":"Yamano-Adachi Noriko"},{"name":"Ogata Norichika"},{"name":"Tanaka Sho"},{"name":"Onitsuka Masayoshi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"Yamano-Adachi Noriko"},{"name":"Ogata Norichika"},{"name":"Tanaka Sho"},{"name":"鬼塚 正義"},{"name":"大政 健史"}]},"publication_date":"2019-07-11","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"volume":"Vol.129","number":"No.1","starting_page":"121","ending_page":"128","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2019.06.012"],"issn":["1389-1723"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:11, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219004"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/30580968","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-85058714330&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=350850","label":"url"}],"paper_title":{"en":"Secretory leakage of IgG1 aggregates from recombinant Chinese hamster ovary cells","ja":"Secretory leakage of IgG1 aggregates from recombinant Chinese hamster ovary cells"},"authors":{"en":[{"name":"Onitsuka Masayoshi"},{"name":"Kadoya Yukinori"},{"name":"Omasa Takeshi"}],"ja":[{"name":"鬼塚 正義"},{"name":"⻆屋 行紀"},{"name":"大政 健史"}]},"description":{"en":"Aggregation of therapeutic antibodies is one of the most important issues to be resolved in manufacturing processes because of reduced efficacy and immunogenicity. Despite aggregation studies in vitro, little is known about the aggregation mechanism in cell culture processes. In this study, we investigated the process of aggregate formation of IgG1 antibodies during the culture of Chinese hamster ovary (CHO) cells to determine how aggregation occurs. A recombinant CHO cell line was cultivated in a bioreactor, and purified IgG1 from daily culture supernatants was analyzed by size exclusion chromatography. We found a linear correlation between the peak plots of IgG1 by-products, dimeric and aggregated IgG1, and integrated viable cell density, indicating that these by-products were secreted from CHO cells at a constant secretion rate. In addition, aggregate formation was not reproduced in pseudo-culture experiments, and the solution structures of intracellular and extracellular IgG1 aggregates were similar. These results support the concept of secretory leakage of IgG1 by-products. Secreted aggregates appeared to be in an alternatively folded state, which can pass through the protein quality control system in mammalian cells.","ja":"Aggregation of therapeutic antibodies is one of the most important issues to be resolved in manufacturing processes because of reduced efficacy and immunogenicity. Despite aggregation studies in vitro, little is known about the aggregation mechanism in cell culture processes. In this study, we investigated the process of aggregate formation of IgG1 antibodies during the culture of Chinese hamster ovary (CHO) cells to determine how aggregation occurs. A recombinant CHO cell line was cultivated in a bioreactor, and purified IgG1 from daily culture supernatants was analyzed by size exclusion chromatography. We found a linear correlation between the peak plots of IgG1 by-products, dimeric and aggregated IgG1, and integrated viable cell density, indicating that these by-products were secreted from CHO cells at a constant secretion rate. In addition, aggregate formation was not reproduced in pseudo-culture experiments, and the solution structures of intracellular and extracellular IgG1 aggregates were similar. These results support the concept of secretory leakage of IgG1 by-products. Secreted aggregates appeared to be in an alternatively folded state, which can pass through the protein quality control system in mammalian cells."},"publication_date":"2019-06","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"volume":"Vol.127","number":"No.6","starting_page":"752","ending_page":"757","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2018.11.015"],"issn":["1347-4421"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:12, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219005"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/30637508","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-85060048909&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=350846","label":"url"}],"paper_title":{"en":"Secretion analysis of intracellular difficult-to-express immunoglobulin G (IgG) in Chinese hamster ovary (CHO) cells","ja":"Secretion analysis of intracellular difficult-to-express immunoglobulin G (IgG) in Chinese hamster ovary (CHO) cells"},"authors":{"en":[{"name":"Kaneyoshi Kohei"},{"name":"Kuroda Kouki"},{"name":"Uchiyama Keiji"},{"name":"Onitsuka Masayoshi"},{"name":"Yamano-Adachi Noriko"},{"name":"Koga Yuichi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"Kaneyoshi Kohei"},{"name":"Kuroda Kouki"},{"name":"内山 圭司"},{"name":"鬼塚 正義"},{"name":"Yamano-Adachi Noriko"},{"name":"Koga Yuichi"},{"name":"大政 健史"}]},"description":{"en":"The Chinese hamster ovary (CHO) cell line is the most widely used host cell for therapeutic antibody production. Although its productivity has been improved by various strategies to satisfy the growing global demand, some difficult-to-express (DTE) antibodies remain at low secretion levels. To improve the production of various therapeutic antibodies, it is necessary to determine possible rate-limiting steps in DTE antibody secretion in comparison with other high IgG producers. Here, we analyzed the protein secretion process in CHO cells producing the DTE immunoglobulin G (IgG) infliximab. The results from chase assays using a translation inhibitor revealed that infliximab secretion could be nearly completed within 2 h, at which time the cells still retained about 40% of heavy chains and 65% of light chains. Using fluorescent microscopy, we observed that these IgG chains remained in the endoplasmic reticulum and Golgi apparatus. The cells inefficiently form fully assembled heterodimer IgG by making LC aggregates, which may be the most serious bottleneck in the production of DTE infliximab compared with other IgG high producers. Our study could contribute to establish the common strategy for constructing DTE high-producer cells on the basis of rate-limiting step analysis.","ja":"The Chinese hamster ovary (CHO) cell line is the most widely used host cell for therapeutic antibody production. Although its productivity has been improved by various strategies to satisfy the growing global demand, some difficult-to-express (DTE) antibodies remain at low secretion levels. To improve the production of various therapeutic antibodies, it is necessary to determine possible rate-limiting steps in DTE antibody secretion in comparison with other high IgG producers. Here, we analyzed the protein secretion process in CHO cells producing the DTE immunoglobulin G (IgG) infliximab. The results from chase assays using a translation inhibitor revealed that infliximab secretion could be nearly completed within 2 h, at which time the cells still retained about 40% of heavy chains and 65% of light chains. Using fluorescent microscopy, we observed that these IgG chains remained in the endoplasmic reticulum and Golgi apparatus. The cells inefficiently form fully assembled heterodimer IgG by making LC aggregates, which may be the most serious bottleneck in the production of DTE infliximab compared with other IgG high producers. Our study could contribute to establish the common strategy for constructing DTE high-producer cells on the basis of rate-limiting step analysis."},"publication_date":"2019-02","publication_name":{"en":"Cytotechnology","ja":"Cytotechnology"},"volume":"Vol.71","number":"No.1","starting_page":"305","ending_page":"316","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1007/s10616-018-0286-5"],"issn":["0920-9069"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:13, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219006"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/30017708","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=342965","label":"url"}],"paper_title":{"en":"Analysis of intracellular IgG secretion in Chinese hamster ovary cells to improve IgG production.","ja":"Analysis of intracellular IgG secretion in Chinese hamster ovary cells to improve IgG production."},"authors":{"en":[{"name":"Kaneyoshi Kohei"},{"name":"Uchiyama Keiji"},{"name":"Onitsuka Masayoshi"},{"name":"Yamano Noriko"},{"name":"Koga Yuichi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"Kaneyoshi Kohei"},{"name":"内山 圭司"},{"name":"鬼塚 正義"},{"name":"山野 範子"},{"name":"Koga Yuichi"},{"name":"大政 健史"}]},"description":{"en":"The production of biopharmaceutical immunoglobulin G (IgG) using cultured mammalian cells, especially Chinese hamster ovary (CHO) cells is well established and has been markedly improved through the modification of cells and cell culture engineering technologies. The establishment of high-production cell lines remains a challenge. The intracellular secretion of IgG has been investigated to identify and solve the rate-limiting steps in antibody production. However, strategies that regulate the expression of proteins that are related to antibody secretory pathway have not consistently improved their production. In this study, key features and limitations of the antibody secretion process in recombinant CHO cells were analyzed to develop more efficient approaches for establishing high-production cells. By chase assay with protein translation inhibitors, IgG secretion reached a plateau when at least 20% of IgG remained in the cells. The secretion kinetics and retention ratio of IgG varied between IgG subclasses (two types of IgG1 and an IgG3 subclass). Immunofluorescent microscopy and size exclusion chromatography showed that the remaining intracellular IgG localized mainly within the endoplasmic reticulum (ER) and less with the cis-Golgi network, despite the formation of fully assembled IgG. These results show that remaining intracellular IgG is a target for enhancing antibody secretion, even in high-production CHO cells.","ja":"The production of biopharmaceutical immunoglobulin G (IgG) using cultured mammalian cells, especially Chinese hamster ovary (CHO) cells is well established and has been markedly improved through the modification of cells and cell culture engineering technologies. The establishment of high-production cell lines remains a challenge. The intracellular secretion of IgG has been investigated to identify and solve the rate-limiting steps in antibody production. However, strategies that regulate the expression of proteins that are related to antibody secretory pathway have not consistently improved their production. In this study, key features and limitations of the antibody secretion process in recombinant CHO cells were analyzed to develop more efficient approaches for establishing high-production cells. By chase assay with protein translation inhibitors, IgG secretion reached a plateau when at least 20% of IgG remained in the cells. The secretion kinetics and retention ratio of IgG varied between IgG subclasses (two types of IgG1 and an IgG3 subclass). Immunofluorescent microscopy and size exclusion chromatography showed that the remaining intracellular IgG localized mainly within the endoplasmic reticulum (ER) and less with the cis-Golgi network, despite the formation of fully assembled IgG. These results show that remaining intracellular IgG is a target for enhancing antibody secretion, even in high-production CHO cells."},"publication_date":"2019-01","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"volume":"Vol.127","number":"No.1","starting_page":"107","ending_page":"113","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2018.06.018"],"issn":["1347-4421"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:14, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219007"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/29970568","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-85049804969&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=348369","label":"url"}],"paper_title":{"en":"Construction of Anti-HER2 Recombinants as Targeting Modules for a Drug-delivery System Against HER2-positive Cells","ja":"Construction of Anti-HER2 Recombinants as Targeting Modules for a Drug-delivery System Against HER2-positive Cells"},"authors":{"en":[{"name":"Tang Qing"},{"name":"Onitsuka Masayoshi"},{"name":"Tabata Atsushi"},{"name":"Tomoyasu Toshifumi"},{"name":"Nagamune Hideaki"}],"ja":[{"name":"唐 卿"},{"name":"鬼塚 正義"},{"name":"田端 厚之"},{"name":"友安 俊文"},{"name":"長宗 秀明"}]},"description":{"en":"Recombinant antibodies have been investigated and used in applications such as targeting modules of drug-delivery systems (DDS) against cancers. This study aimed to prepare recombinant antibodies against HER2, containing sortase A (SrtA) recognition sequence, that are applicable as targeting modules in DDS after linkage with the drug-carrier containing oligoglycine-acceptor peptide by SrtA transpeptidation. The recombinant trastuzumab fragment antibodies (scFvs and Fab) with the SrtA-recognition motif (LPXTG) at their C-terminal were constructed and expressed in Escherichia coli and Chinese hamster ovary (CHO) cells, respectively. The reactivity of the purified recombinant antibodies towards HER2-expressing cells was also evaluated via immunofluorescent staining. Fab demonstrated higher yield and purity and better reactivity towards HER2-expressing cells (HCT-15 and HeLa) when compared to scFvs. The CHO expression system possesses superior yield and purity when compared to the E. coli expression system with respect to the preparation of recombinant antibodies applicable in targeting modules for DDS (DDS-TM). Moreover, a Fab variant prepared in this study demonstrated the potential to be a DDS-TM against HER2-expressing cancer cells.","ja":"Recombinant antibodies have been investigated and used in applications such as targeting modules of drug-delivery systems (DDS) against cancers. This study aimed to prepare recombinant antibodies against HER2, containing sortase A (SrtA) recognition sequence, that are applicable as targeting modules in DDS after linkage with the drug-carrier containing oligoglycine-acceptor peptide by SrtA transpeptidation. The recombinant trastuzumab fragment antibodies (scFvs and Fab) with the SrtA-recognition motif (LPXTG) at their C-terminal were constructed and expressed in Escherichia coli and Chinese hamster ovary (CHO) cells, respectively. The reactivity of the purified recombinant antibodies towards HER2-expressing cells was also evaluated via immunofluorescent staining. Fab demonstrated higher yield and purity and better reactivity towards HER2-expressing cells (HCT-15 and HeLa) when compared to scFvs. The CHO expression system possesses superior yield and purity when compared to the E. coli expression system with respect to the preparation of recombinant antibodies applicable in targeting modules for DDS (DDS-TM). Moreover, a Fab variant prepared in this study demonstrated the potential to be a DDS-TM against HER2-expressing cancer cells."},"publication_date":"2018-07","publication_name":{"en":"Anticancer Research","ja":"Anticancer Research"},"volume":"Vol.38","number":"No.7","starting_page":"4319","ending_page":"4325","languages":["eng"],"referee":true,"identifiers":{"doi":["10.21873/anticanres.12731"],"issn":["1791-7530"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:15, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219008"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/29188404","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-85035361000&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=343353","label":"url"}],"paper_title":{"en":"Enhanced IgG1 production by overexpression of nuclear factor kappa B inhibitor zeta (NFKBIZ) in Chinese hamster ovary cells","ja":"Enhanced IgG1 production by overexpression of nuclear factor kappa B inhibitor zeta (NFKBIZ) in Chinese hamster ovary cells"},"authors":{"en":[{"name":"Onitsuka Masayoshi"},{"name":"Kinoshita Yukie"},{"name":"Nishizawa Akitoshi"},{"name":"Tsutsui Tomomi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"鬼塚 正義"},{"name":"木下 幸恵"},{"name":"Nishizawa Akitoshi"},{"name":"Tsutsui Tomomi"},{"name":"大政 健史"}]},"description":{"en":"Several engineering strategies have been employed to improve the production of therapeutic recombinant proteins in Chinese hamster ovary (CHO) cell lines. We have focused on unfolded protein response-based engineering and reported that ATF4 overexpression increases protein production. In this study, transcriptome analysis of ATF4-overexpressed CHO cells was performed using high-coverage expression profiling, to search for another key factor contributing to recombinant protein production. We observed the upregulated expression of transcription factor, nuclear factor (NF)-kappa-B inhibitor zeta (NFKBIZ or Iκbζ), in ATF4-overexpressed cells. A total of 1917 bp of CHO NFKBIZ cDNA was cloned, and two stable cell lines overexpressing NFKBIZ were constructed. We investigated the effects of NFKBIZ on IgG1 production in CHO cells. Although the two stable cell lines, NFKBIZ-A and -B, had the opposite phenotypes in cell growth, the specific IgG1 production rate of both cell lines was enhanced by 1.2-1.4-fold. In the NFKBIZ-A cell line, the synergistic effect between enhanced viable cell density and improved specific IgG1 production rate brought about a large increase in the final IgG1 titer. Luciferase-based NF-κB signaling assay results suggest that altered p50/p50 signaling seems to be due to the opposite phenotypes in cell growth. No difference was observed in the translational levels and intracellular assembly states of IgG1 between mock and two NFKBIZ cell lines, indicating that the secretion machinery of correctly folded IgG1 was enhanced in NFKBIZ-overexpressing cell lines.","ja":"Several engineering strategies have been employed to improve the production of therapeutic recombinant proteins in Chinese hamster ovary (CHO) cell lines. We have focused on unfolded protein response-based engineering and reported that ATF4 overexpression increases protein production. In this study, transcriptome analysis of ATF4-overexpressed CHO cells was performed using high-coverage expression profiling, to search for another key factor contributing to recombinant protein production. We observed the upregulated expression of transcription factor, nuclear factor (NF)-kappa-B inhibitor zeta (NFKBIZ or Iκbζ), in ATF4-overexpressed cells. A total of 1917 bp of CHO NFKBIZ cDNA was cloned, and two stable cell lines overexpressing NFKBIZ were constructed. We investigated the effects of NFKBIZ on IgG1 production in CHO cells. Although the two stable cell lines, NFKBIZ-A and -B, had the opposite phenotypes in cell growth, the specific IgG1 production rate of both cell lines was enhanced by 1.2-1.4-fold. In the NFKBIZ-A cell line, the synergistic effect between enhanced viable cell density and improved specific IgG1 production rate brought about a large increase in the final IgG1 titer. Luciferase-based NF-κB signaling assay results suggest that altered p50/p50 signaling seems to be due to the opposite phenotypes in cell growth. No difference was observed in the translational levels and intracellular assembly states of IgG1 between mock and two NFKBIZ cell lines, indicating that the secretion machinery of correctly folded IgG1 was enhanced in NFKBIZ-overexpressing cell lines."},"publication_date":"2018-04","publication_name":{"en":"Cytotechnology","ja":"Cytotechnology"},"volume":"Vol.70","number":"No.2","starting_page":"675","ending_page":"685","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1007/s10616-017-0170-8"],"issn":["0920-9069"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:16, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219009"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/26850366","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-84956706908&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=307447","label":"url"}],"paper_title":{"en":"Increased recombinant protein production owing to expanded opportunities for vector integration in high chromosome number Chinese hamster ovary cells","ja":"Increased recombinant protein production owing to expanded opportunities for vector integration in high chromosome number Chinese hamster ovary cells"},"authors":{"en":[{"name":"Yamano Noriko"},{"name":"Takahashi Mai"},{"name":"Seyed Mohammad Ali Haghparast"},{"name":"Onitsuka Masayoshi"},{"name":"Kumamoto Toshitaka"},{"name":"Frank Jana"},{"name":"Omasa Takeshi"}],"ja":[{"name":"山野 範子"},{"name":"Takahashi Mai"},{"name":"Seyed Mohammad Ali Haghparast"},{"name":"鬼塚 正義"},{"name":"Kumamoto Toshitaka"},{"name":"フランク ヤナ"},{"name":"大政 健史"}]},"description":{"en":"Chromosomal instability is a characteristic of Chinese hamster ovary (CHO) cells. Cultures of these cells gradually develop heterogeneity even if established from a single cell clone. We isolated cells containing different numbers of chromosomes from a CHO-DG44-based human granulocyte-macrophage colony stimulating factor (hGM-CSF)-producing cell line and found that high chromosome number cells showed higher hGM-CSF productivity. Therefore, we focused on the relationship between chromosome aneuploidy of CHO cells and high recombinant protein-producing cell lines. Distribution and stability of chromosomes were examined in CHO-DG44 cells, and two cell lines expressing different numbers of chromosomes were isolated from the original CHO-DG44 cell line to investigate the effect of aneuploid cells on recombinant protein production. Both cell lines were stably transfected with a vector that expresses immunoglobulin G3 (IgG3), and specific antibody production rates were compared. Cells containing more than 30 chromosomes had higher specific antibody production rates than those with normal chromosome number. Single cell analysis of enhanced green fluorescent protein (Egfp)-gene transfected cells revealed that increased GFP expression was relative to the number of gene integration sites rather than the difference in chromosome numbers or vector locations. Our results suggest that CHO cells with high numbers of chromosomes contain more sites for vector integration, a characteristic that could be advantageous in biopharmaceutical production.","ja":"Chromosomal instability is a characteristic of Chinese hamster ovary (CHO) cells. Cultures of these cells gradually develop heterogeneity even if established from a single cell clone. We isolated cells containing different numbers of chromosomes from a CHO-DG44-based human granulocyte-macrophage colony stimulating factor (hGM-CSF)-producing cell line and found that high chromosome number cells showed higher hGM-CSF productivity. Therefore, we focused on the relationship between chromosome aneuploidy of CHO cells and high recombinant protein-producing cell lines. Distribution and stability of chromosomes were examined in CHO-DG44 cells, and two cell lines expressing different numbers of chromosomes were isolated from the original CHO-DG44 cell line to investigate the effect of aneuploid cells on recombinant protein production. Both cell lines were stably transfected with a vector that expresses immunoglobulin G3 (IgG3), and specific antibody production rates were compared. Cells containing more than 30 chromosomes had higher specific antibody production rates than those with normal chromosome number. Single cell analysis of enhanced green fluorescent protein (Egfp)-gene transfected cells revealed that increased GFP expression was relative to the number of gene integration sites rather than the difference in chromosome numbers or vector locations. Our results suggest that CHO cells with high numbers of chromosomes contain more sites for vector integration, a characteristic that could be advantageous in biopharmaceutical production."},"publication_date":"2016-08","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"volume":"Vol.122","number":"No.2","starting_page":"226","ending_page":"231","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2016.01.002"],"issn":["1389-1723"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:17, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219010"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/26803706","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-85027930962&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=311612","label":"url"}],"paper_title":{"en":"Metabolic analysis of antibody producing Chinese hamster ovary cell culture under different stresses conditions.","ja":"Metabolic analysis of antibody producing Chinese hamster ovary cell culture under different stresses conditions."},"authors":{"en":[{"name":"Badsha Md Bahadur"},{"name":"Kurata Hiroyuki"},{"name":"Onitsuka Masayoshi"},{"name":"Oga Takushi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"Badsha Md Bahadur"},{"name":"Kurata Hiroyuki"},{"name":"鬼塚 正義"},{"name":"Oga Takushi"},{"name":"大政 健史"}]},"description":{"en":"Chinese hamster ovary (CHO) cells are commonly used as the host cell lines concerning their ability to produce therapeutic proteins with complex post-translational modifications. In this study, we have investigated the time course extra- and intracellular metabolome data of the CHO-K1 cell line, under a control and stress conditions. The addition of NaCl and trehalose greatly suppressed cell growth, where the maximum viable cell density of NaCl and trehalose cultures were 2.2-fold and 2.8-fold less than that of a control culture. Contrariwise, the antibody production of both the NaCl and trehalose cultures was sustained for a longer time to surpass that of the control culture. The NaCl and trehalose cultures showed relatively similar dynamics of cell growth, antibody production, and substrate/product concentrations, while they indicated different dynamics from the control culture. The principal component analysis of extra- and intracellular metabolome dynamics indicated that their dynamic behaviors were consistent with biological functions. The qualitative pattern matching classification and hierarchical clustering analyses for the intracellular metabolome identified the metabolite clusters whose dynamic behaviors depend on NaCl and trehalose. The volcano plot revealed several reporter metabolites whose dynamics greatly change between in the NaCl and trehalose cultures. The elastic net identified some critical, intracellular metabolites that are distinct between the NaCl and trehalose. While a relatively small number of intracellular metabolites related to the cell growth, glucose, glutamine, lactate and ammonium ion concentrations, the mechanism of antibody production was suggested to be very complicated or not to be explained by elastic net regression analysis.","ja":"Chinese hamster ovary (CHO) cells are commonly used as the host cell lines concerning their ability to produce therapeutic proteins with complex post-translational modifications. In this study, we have investigated the time course extra- and intracellular metabolome data of the CHO-K1 cell line, under a control and stress conditions. The addition of NaCl and trehalose greatly suppressed cell growth, where the maximum viable cell density of NaCl and trehalose cultures were 2.2-fold and 2.8-fold less than that of a control culture. Contrariwise, the antibody production of both the NaCl and trehalose cultures was sustained for a longer time to surpass that of the control culture. The NaCl and trehalose cultures showed relatively similar dynamics of cell growth, antibody production, and substrate/product concentrations, while they indicated different dynamics from the control culture. The principal component analysis of extra- and intracellular metabolome dynamics indicated that their dynamic behaviors were consistent with biological functions. The qualitative pattern matching classification and hierarchical clustering analyses for the intracellular metabolome identified the metabolite clusters whose dynamic behaviors depend on NaCl and trehalose. The volcano plot revealed several reporter metabolites whose dynamics greatly change between in the NaCl and trehalose cultures. The elastic net identified some critical, intracellular metabolites that are distinct between the NaCl and trehalose. While a relatively small number of intracellular metabolites related to the cell growth, glucose, glutamine, lactate and ammonium ion concentrations, the mechanism of antibody production was suggested to be very complicated or not to be explained by elastic net regression analysis."},"publication_date":"2016-01-20","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2015.12.013"],"issn":["1347-4421"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:18, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219011"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/26108159","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=311611","label":"url"}],"paper_title":{"en":"Improved gene amplification by cell-cycle engineering combined with the Cre-loxP system in Chinese hamster ovary cells.","ja":"Improved gene amplification by cell-cycle engineering combined with the Cre-loxP system in Chinese hamster ovary cells."},"authors":{"en":[{"name":"Matsuyama Rima"},{"name":"Tsutsui Tomomi"},{"name":"Lee Kyoung Ho"},{"name":"Onitsuka Masayoshi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"Matsuyama Rima"},{"name":"Tsutsui Tomomi"},{"name":"Lee Kyoung Ho"},{"name":"鬼塚 正義"},{"name":"大政 健史"}]},"description":{"en":"The dihydrofolate reductase gene amplification system is widely used in Chinese hamster ovary (CHO) cells for the industrial production of therapeutic proteins. To enhance the efficiency of conventional gene amplification systems, we previously presented a novel method using cell-cycle checkpoint engineering. Here, we constructed high-producing and stable cells by the conditional expression of mutant cell division cycle 25 homolog B (CDC25B) using the Cre-loxP system. A bispecific antibody-producing CHO DG44-derived cell line was transfected with floxed mutant CDC25B. After inducing gene amplification in the presence of 250 nM methotrexate, mutant CDC25B sequence was removed by Cre recombinase protein expression. Overexpression of the floxed mutant CDC25B significantly enhanced the efficiency of transgene amplification and productivity. Moreover, the specific production rate of the isolated clone CHO Cre-1 and Cre-2 were approximately 11-fold and 15-fold higher than that of mock-transfected clone CHO Mock-S. Chromosomal aneuploidy was increased by mutant CDC25B overexpression, but Cre-1 and Cre-2 did not show any changes in chromosome number during long-term cultivation, as is the case with CHO Mock-S. Our results suggest that high-producing and stable cells can be constructed by conditionally controlling a cell-cycle checkpoint integrated in conventional gene amplification systems.","ja":"The dihydrofolate reductase gene amplification system is widely used in Chinese hamster ovary (CHO) cells for the industrial production of therapeutic proteins. To enhance the efficiency of conventional gene amplification systems, we previously presented a novel method using cell-cycle checkpoint engineering. Here, we constructed high-producing and stable cells by the conditional expression of mutant cell division cycle 25 homolog B (CDC25B) using the Cre-loxP system. A bispecific antibody-producing CHO DG44-derived cell line was transfected with floxed mutant CDC25B. After inducing gene amplification in the presence of 250 nM methotrexate, mutant CDC25B sequence was removed by Cre recombinase protein expression. Overexpression of the floxed mutant CDC25B significantly enhanced the efficiency of transgene amplification and productivity. Moreover, the specific production rate of the isolated clone CHO Cre-1 and Cre-2 were approximately 11-fold and 15-fold higher than that of mock-transfected clone CHO Mock-S. Chromosomal aneuploidy was increased by mutant CDC25B overexpression, but Cre-1 and Cre-2 did not show any changes in chromosome number during long-term cultivation, as is the case with CHO Mock-S. Our results suggest that high-producing and stable cells can be constructed by conditionally controlling a cell-cycle checkpoint integrated in conventional gene amplification systems."},"publication_date":"2015-06-21","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"volume":"Vol.120","number":"No.6","starting_page":"701","ending_page":"708","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2015.04.009"],"issn":["1347-4421"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:19, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219012"},"force":{"see_also":[{"@id":"http://ci.nii.ac.jp/naid/130005061978/","label":"url"},{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/25817810","label":"url"},{"@id":"https://cir.nii.ac.jp/crid/1390282679440670976/","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-84926366827&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=284933","label":"url"}],"paper_title":{"en":"Effect of polyphenols on reactive oxygen species production and cell growth of human dermal fibroblasts after irradiation with ultraviolet-A light","ja":"Effect of polyphenols on reactive oxygen species production and cell growth of human dermal fibroblasts after irradiation with ultraviolet-A light"},"authors":{"en":[{"name":"Shirai Akihiro"},{"name":"Onitsuka Masayoshi"},{"name":"Maseda Hideaki"},{"name":"Omasa Takeshi"}],"ja":[{"name":"白井 昭博"},{"name":"鬼塚 正義"},{"name":"間世田 英明"},{"name":"大政 健史"}]},"description":{"en":"Ultraviolet-A (UV-A) can damage microbes by generating reactive oxygen species (ROS), singlet oxygen, superoxides, hydrogen peroxide and hydroxyl radicals. These species readily react with lipids, proteins, DNA and other constituents of cells, leading to oxidative deterioration and the eventual death of the microbe. However, the oxidative ability of these reactive species also harms the viability of mammalian cells such as fibroblasts and keratinocytes, as they cause both acute and chronic damage, photo-aging, and photo-carcinogenesis. This study describes a UV-A treatment that does not affect the viability or growth of human neonate dermal fibroblasts, as determined by examining the post-irradiation cell density after the addition of polyphenols as antioxidants. The results demonstrate the possible wide applicability of UV-A sterilization. The potency of polyphenols for attenuating UV-A-induced ROS generation in cells was tested using (+)-catechin hydrate, (-)- epigallocatechin gallate hydrate, morin hydrate, quercetin hydrate and resveratrol. The lowest concentration of polyphenols required to reduce ROS by 50% in cells upon exposure to a dose of 15 J cm-2 was determined and defined as its IC50. Pre-treatment with morin hydrate at its IC50 allowed cells irradiated with 5.0 J cm-2 UV-A to recover to the level of the specific growth rate of cells incubated without UV-A irradiation. However, the growth rate of cells exposed to 15 J cm-2 UV-A irradiation was scarcely influenced by co-incubation with morin hydrate; this dose of UV-A also suppressed cell growthcompletely in the absence of morin hydrate, although co-incubation resulted in no decrease in cell viability. This study demonstrates the potential of polyphenols for protecting both the viability of cells and their ability to proliferate from damage caused by UV-A-irradiation.","ja":"Ultraviolet-A (UV-A) can damage microbes by generating reactive oxygen species (ROS), singlet oxygen, superoxides, hydrogen peroxide and hydroxyl radicals. These species readily react with lipids, proteins, DNA and other constituents of cells, leading to oxidative deterioration and the eventual death of the microbe. However, the oxidative ability of these reactive species also harms the viability of mammalian cells such as fibroblasts and keratinocytes, as they cause both acute and chronic damage, photo-aging, and photo-carcinogenesis. This study describes a UV-A treatment that does not affect the viability or growth of human neonate dermal fibroblasts, as determined by examining the post-irradiation cell density after the addition of polyphenols as antioxidants. The results demonstrate the possible wide applicability of UV-A sterilization. The potency of polyphenols for attenuating UV-A-induced ROS generation in cells was tested using (+)-catechin hydrate, (-)- epigallocatechin gallate hydrate, morin hydrate, quercetin hydrate and resveratrol. The lowest concentration of polyphenols required to reduce ROS by 50% in cells upon exposure to a dose of 15 J cm-2 was determined and defined as its IC50. Pre-treatment with morin hydrate at its IC50 allowed cells irradiated with 5.0 J cm-2 UV-A to recover to the level of the specific growth rate of cells incubated without UV-A irradiation. However, the growth rate of cells exposed to 15 J cm-2 UV-A irradiation was scarcely influenced by co-incubation with morin hydrate; this dose of UV-A also suppressed cell growthcompletely in the absence of morin hydrate, although co-incubation resulted in no decrease in cell viability. This study demonstrates the potential of polyphenols for protecting both the viability of cells and their ability to proliferate from damage caused by UV-A-irradiation."},"publication_date":"2015-03-10","publication_name":{"en":"Biocontrol Science","ja":"Biocontrol Science"},"volume":"Vol.20","number":"No.1","starting_page":"27","ending_page":"33","languages":["eng"],"referee":true,"identifiers":{"doi":["10.4265/bio.20.27"],"issn":["1884-0205"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:20, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219013"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/25548123","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=311609","label":"url"}],"paper_title":{"en":"Rapid evaluation of N-glycosylation status of antibodies with chemiluminescent lectin-binding assay.","ja":"Rapid evaluation of N-glycosylation status of antibodies with chemiluminescent lectin-binding assay."},"authors":{"en":[{"name":"Onitsuka Masayoshi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"鬼塚 正義"},{"name":"大政 健史"}]},"description":{"en":"We constructed an assay system for the rapid detection of the glycosylation status of antibodies with a chemiluminescence-based lectin-binding assay, and investigated the glycosylation dynamics during the culture of recombinant Chinese hamster ovary cells. This rapid detection system is applicable to the high-throughput evaluation of therapeutic glycoproteins.","ja":"We constructed an assay system for the rapid detection of the glycosylation status of antibodies with a chemiluminescence-based lectin-binding assay, and investigated the glycosylation dynamics during the culture of recombinant Chinese hamster ovary cells. This rapid detection system is applicable to the high-throughput evaluation of therapeutic glycoproteins."},"publication_date":"2014-12-23","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"volume":"Vol.120","number":"No.1","starting_page":"107","ending_page":"110","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2014.11.015"],"issn":["1347-4421"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:21, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219014"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/25517309","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=311610","label":"url"}],"paper_title":{"en":"Rearranging the domain order of a diabody-based IgG-like bispecific antibody enhances its antitumor activity and improves its degradation resistance and pharmacokinetics.","ja":"Rearranging the domain order of a diabody-based IgG-like bispecific antibody enhances its antitumor activity and improves its degradation resistance and pharmacokinetics."},"authors":{"en":[{"name":"Asano Ryutaro"},{"name":"Shimomura Ippei"},{"name":"Konno Shota"},{"name":"Ito Akiko"},{"name":"Masakari Yosuke"},{"name":"Orimo Ryota"},{"name":"Taki Shintaro"},{"name":"Arai Kyoko"},{"name":"Ogata Hiromi"},{"name":"Okada Mai"},{"name":"Furumoto Shozo"},{"name":"Onitsuka Masayoshi"},{"name":"Omasa Takeshi"},{"name":"Hayashi Hiroki"},{"name":"Katayose Yu"},{"name":"Unno Michiaki"},{"name":"Kudo Toshio"},{"name":"Umetsu Mitsuo"},{"name":"Kumagai Izumi"}],"ja":[{"name":"Asano Ryutaro"},{"name":"Shimomura Ippei"},{"name":"Konno Shota"},{"name":"Ito Akiko"},{"name":"Masakari Yosuke"},{"name":"Orimo Ryota"},{"name":"Taki Shintaro"},{"name":"Arai Kyoko"},{"name":"Ogata Hiromi"},{"name":"Okada Mai"},{"name":"Furumoto Shozo"},{"name":"鬼塚 正義"},{"name":"大政 健史"},{"name":"Hayashi Hiroki"},{"name":"Katayose Yu"},{"name":"Unno Michiaki"},{"name":"Kudo Toshio"},{"name":"Umetsu Mitsuo"},{"name":"Kumagai Izumi"}]},"description":{"en":"One approach to creating more beneficial therapeutic antibodies is to develop bispecific antibodies (bsAbs), particularly IgG-like formats with tetravalency, which may provide several advantages such as multivalent binding to each target antigen. Although the effects of configuration and antibody-fragment type on the function of IgG-like bsAbs have been studied, there have been only a few detailed studies of the influence of the variable fragment domain order. Here, we prepared four types of hEx3-scDb-Fc, IgG-like bsAbs, built from a single-chain hEx3-Db (humanized bispecific diabody [bsDb] that targets epidermal growth factor receptor and CD3), to investigate the influence of domain order and fusion manner on the function of a bsDb with an Fc fusion format. Higher cytotoxicities were observed with hEx3-scDb-Fcs with a variable light domain (VL)-variable heavy domain (VH) order (hEx3-scDb-Fc-LHs) compared with a VH-VL order, indicating that differences in the Fc fusion manner do not affect bsDb activity. In addition, flow cytometry suggested that the higher cytotoxicities of hEx3-scDb-Fc-LH may be attributable to structural superiority in cross-linking. Interestingly, enhanced degradation resistance and prolonged in vivo half-life were also observed with hEx3-scDb-Fc-LH. hEx3-scDb-Fc-LH and its IgG2 variant exhibited intense in vivo antitumor effects, suggesting that Fc-mediated effector functions are dispensable for effective anti-tumor activities, which may cause fewer side effects. Our results show that merely rearranging the domain order of IgG-like bsAbs can enhance not only their antitumor activity, but also their degradation resistance and in vivo half-life, and that hEx3-scDb-Fc-LHs are potent candidates for next-generation therapeutic antibodies.","ja":"One approach to creating more beneficial therapeutic antibodies is to develop bispecific antibodies (bsAbs), particularly IgG-like formats with tetravalency, which may provide several advantages such as multivalent binding to each target antigen. Although the effects of configuration and antibody-fragment type on the function of IgG-like bsAbs have been studied, there have been only a few detailed studies of the influence of the variable fragment domain order. Here, we prepared four types of hEx3-scDb-Fc, IgG-like bsAbs, built from a single-chain hEx3-Db (humanized bispecific diabody [bsDb] that targets epidermal growth factor receptor and CD3), to investigate the influence of domain order and fusion manner on the function of a bsDb with an Fc fusion format. Higher cytotoxicities were observed with hEx3-scDb-Fcs with a variable light domain (VL)-variable heavy domain (VH) order (hEx3-scDb-Fc-LHs) compared with a VH-VL order, indicating that differences in the Fc fusion manner do not affect bsDb activity. In addition, flow cytometry suggested that the higher cytotoxicities of hEx3-scDb-Fc-LH may be attributable to structural superiority in cross-linking. Interestingly, enhanced degradation resistance and prolonged in vivo half-life were also observed with hEx3-scDb-Fc-LH. hEx3-scDb-Fc-LH and its IgG2 variant exhibited intense in vivo antitumor effects, suggesting that Fc-mediated effector functions are dispensable for effective anti-tumor activities, which may cause fewer side effects. Our results show that merely rearranging the domain order of IgG-like bsAbs can enhance not only their antitumor activity, but also their degradation resistance and in vivo half-life, and that hEx3-scDb-Fc-LHs are potent candidates for next-generation therapeutic antibodies."},"publication_date":"2014-10-30","publication_name":{"en":"mAbs","ja":"mAbs"},"volume":"Vol.6","number":"No.5","starting_page":"1243","ending_page":"1254","languages":["eng"],"referee":true,"identifiers":{"doi":["10.4161/mabs.29445"],"issn":["1942-0870"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:22, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219015"},"force":{"see_also":[{"@id":"http://ci.nii.ac.jp/naid/110009823142/","label":"url"},{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/24315529","label":"url"},{"@id":"https://cir.nii.ac.jp/crid/1522262180374430720/","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-84897055074&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=276959","label":"url"}],"paper_title":{"en":"Trehalose suppresses antibody aggregation during the culture of Chinese hamster ovary cells","ja":"Trehalose suppresses antibody aggregation during the culture of Chinese hamster ovary cells"},"authors":{"en":[{"name":"Onitsuka Masayoshi"},{"name":"Tatsuzawa Miki"},{"name":"Asano Ryutaro"},{"name":"Kumagai Izumi"},{"name":"Shirai Akihiro"},{"name":"Maseda Hideaki"},{"name":"Omasa Takeshi"}],"ja":[{"name":"鬼塚 正義"},{"name":"Tatsuzawa Miki"},{"name":"Asano Ryutaro"},{"name":"Kumagai Izumi"},{"name":"白井 昭博"},{"name":"間世田 英明"},{"name":"大政 健史"}]},"description":{"en":"The aggregation of therapeutic antibodies during the manufacturing process is problematic because of the potential risks posed by the aggregates, such as an unexpected immune response. One of the hallmark effects of trehalose, a disaccharide consisting of two alpha-glucose units, is as a chemical chaperone with anti-aggregation activity. In this study, Chinese hamster ovary (CHO) cell line producing a diabody-type bispecific antibody were cultured in medium containing trehalose and the aggregation of the secreted proteins during the culture process was analyzed. An analysis of the various forms of the antibody (monomeric, dimeric, and large aggregates) showed that trehalose decreased the relative content of large aggregates by two thirds. The aggregation kinetics indicated that trehalose directly inhibited the polymerization and aggregation steps in a nucleation-dependent aggregation mechanism. Moreover, both specific and volumetric antibody production were increased in CHO cells cultured in trehalose-containing medium. Thus, the addition of trehalose to recombinant CHO cell cultures would offer a practical strategy for quality improvement in the production of therapeutic antibodies.","ja":"The aggregation of therapeutic antibodies during the manufacturing process is problematic because of the potential risks posed by the aggregates, such as an unexpected immune response. One of the hallmark effects of trehalose, a disaccharide consisting of two alpha-glucose units, is as a chemical chaperone with anti-aggregation activity. In this study, Chinese hamster ovary (CHO) cell line producing a diabody-type bispecific antibody were cultured in medium containing trehalose and the aggregation of the secreted proteins during the culture process was analyzed. An analysis of the various forms of the antibody (monomeric, dimeric, and large aggregates) showed that trehalose decreased the relative content of large aggregates by two thirds. The aggregation kinetics indicated that trehalose directly inhibited the polymerization and aggregation steps in a nucleation-dependent aggregation mechanism. Moreover, both specific and volumetric antibody production were increased in CHO cells cultured in trehalose-containing medium. Thus, the addition of trehalose to recombinant CHO cell cultures would offer a practical strategy for quality improvement in the production of therapeutic antibodies."},"publication_date":"2014-05","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"volume":"Vol.117","number":"No.5","starting_page":"632","ending_page":"638","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2013.10.022"],"issn":["1347-4421"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:23, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219016"},"force":{"see_also":[{"@id":"http://id.ndl.go.jp/bib/025469532","label":"url"},{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/24326352","label":"url"},{"@id":"https://cir.nii.ac.jp/crid/1521980705029265664/","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-84897065464&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=276943","label":"url"}],"paper_title":{"en":"Glycosylation analysis of an aggregated antibody produced by Chinese hamster ovary cells in bioreactor culture","ja":"Glycosylation analysis of an aggregated antibody produced by Chinese hamster ovary cells in bioreactor culture"},"authors":{"en":[{"name":"Onitsuka Masayoshi"},{"name":"Kawaguchi Akira"},{"name":"Asano Ryutaro"},{"name":"Kumagai Izumi"},{"name":"Honda Kohsuke"},{"name":"Ohtake Hisao"},{"name":"Omasa Takeshi"}],"ja":[{"name":"鬼塚 正義"},{"name":"Kawaguchi Akira"},{"name":"Asano Ryutaro"},{"name":"Kumagai Izumi"},{"name":"Honda Kohsuke"},{"name":"Ohtake Hisao"},{"name":"大政 健史"}]},"description":{"en":"N-Glycosylation of therapeutic antibodies contributes not only to their biological function, but also to their stability and tendency to aggregate. Here, we investigated the impact of the glycosylation status of an aggregated antibody that accumulated during the bioreactor culture of Chinese hamster ovary cells. High-performance liquid chromatography analysis showed that there was no apparent difference in the glycosylation patterns of monomeric, dimeric, and large aggregated forms of the antibody. In contrast, lectin binding assays, which enable the total amounts of specific sugar residues to be detected, showed that both galactose and fucose residues in dimers and large aggregates were reduced to 70-80% of the amount in monomers. These results strongly suggest that the lack of N-linked oligosaccharides, a result of deglycosylation or aglycosylation, occurred in a proportion of the dimeric and large aggregated components. The present study demonstrates that glycosylation heterogeneities are a potential cause of antibody aggregation in cell culture of Chinese hamster ovary cells, and that the lack of N-glycosylation promotes the formation of dimers and finally results in large aggregates.","ja":"N-Glycosylation of therapeutic antibodies contributes not only to their biological function, but also to their stability and tendency to aggregate. Here, we investigated the impact of the glycosylation status of an aggregated antibody that accumulated during the bioreactor culture of Chinese hamster ovary cells. High-performance liquid chromatography analysis showed that there was no apparent difference in the glycosylation patterns of monomeric, dimeric, and large aggregated forms of the antibody. In contrast, lectin binding assays, which enable the total amounts of specific sugar residues to be detected, showed that both galactose and fucose residues in dimers and large aggregates were reduced to 70-80% of the amount in monomers. These results strongly suggest that the lack of N-linked oligosaccharides, a result of deglycosylation or aglycosylation, occurred in a proportion of the dimeric and large aggregated components. The present study demonstrates that glycosylation heterogeneities are a potential cause of antibody aggregation in cell culture of Chinese hamster ovary cells, and that the lack of N-glycosylation promotes the formation of dimers and finally results in large aggregates."},"publication_date":"2014-05","publication_name":{"en":"Journal of Bioscience and Bioengineering","ja":"Journal of Bioscience and Bioengineering"},"volume":"Vol.117","number":"No.5","starting_page":"639","ending_page":"644","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1016/j.jbiosc.2013.11.001"],"issn":["1389-1723"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:24, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219017"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/23615744","label":"url"},{"@id":"https://www.scopus.com/record/display.url?eid=2-s2.0-84879418366&origin=inward","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=272381","label":"url"}],"paper_title":{"en":"Rapid construction of transgene-amplified CHO cell lines by cell cycle checkpoint engineering","ja":"Rapid construction of transgene-amplified CHO cell lines by cell cycle checkpoint engineering"},"authors":{"en":[{"name":"Kyoung Ho Lee"},{"name":"Onitsuka Masayoshi"},{"name":"Honda Kohsuke"},{"name":"Ohtake Hisao"},{"name":"Omasa Takeshi"}],"ja":[{"name":"Kyoung Ho Lee"},{"name":"鬼塚 正義"},{"name":"Honda Kohsuke"},{"name":"Ohtake Hisao"},{"name":"大政 健史"}]},"description":{"en":"The process of establishing high-producing cell lines for the manufacture of therapeutic proteins is usually both time-consuming and laborious due to the low probability of obtaining high-producing clones from a pool of transfected cells and slow cell growth under the strong selective pressure of screening to identify high-producing clones. We present a novel method to rapidly generate more high-producing cells by accelerating transgene amplification. A small interfering RNA (siRNA) expression vector against ataxia telangiectasia and Rad3 related (ATR), a cell cycle checkpoint kinase, was transfected into Chinese hamster ovary (CHO) cells. The influences of ATR downregulation on gene amplification and the productivity were investigated in CHO cells producing green fluorescent protein (GFP) and secreting monoclonal antibody (mAb). The ATR-downregulated cells showed up to a 6-fold higher ratio of GFP-positive cells than that of the control cell pool. Moreover, the downregulated mAb-producing cells had about a 4-fold higher specific production rate and a 3-fold higher volumetric productivity as compared with the mock cells. ATR-downregulated cells showed a much faster increase in transgene copy numbers during the gene amplification process via methotrexate (MTX) treatment in both GFP- and mAb-producing cells. Our results suggest that a pool of high-producing cells can be more rapidly generated by ATR downregulation as compared with conventional gene amplification by MTX treatment. This novel method may be a promising approach to reduce time and labor in the process of cell line development.","ja":"The process of establishing high-producing cell lines for the manufacture of therapeutic proteins is usually both time-consuming and laborious due to the low probability of obtaining high-producing clones from a pool of transfected cells and slow cell growth under the strong selective pressure of screening to identify high-producing clones. We present a novel method to rapidly generate more high-producing cells by accelerating transgene amplification. A small interfering RNA (siRNA) expression vector against ataxia telangiectasia and Rad3 related (ATR), a cell cycle checkpoint kinase, was transfected into Chinese hamster ovary (CHO) cells. The influences of ATR downregulation on gene amplification and the productivity were investigated in CHO cells producing green fluorescent protein (GFP) and secreting monoclonal antibody (mAb). The ATR-downregulated cells showed up to a 6-fold higher ratio of GFP-positive cells than that of the control cell pool. Moreover, the downregulated mAb-producing cells had about a 4-fold higher specific production rate and a 3-fold higher volumetric productivity as compared with the mock cells. ATR-downregulated cells showed a much faster increase in transgene copy numbers during the gene amplification process via methotrexate (MTX) treatment in both GFP- and mAb-producing cells. Our results suggest that a pool of high-producing cells can be more rapidly generated by ATR downregulation as compared with conventional gene amplification by MTX treatment. This novel method may be a promising approach to reduce time and labor in the process of cell line development."},"publication_date":"2013-04-25","publication_name":{"en":"Applied Microbiology and Biotechnology","ja":"Applied Microbiology and Biotechnology"},"volume":"Vol.97","number":"No.13","starting_page":"5731","ending_page":"5741","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1007/s00253-013-4923-9"],"issn":["1432-0614"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:25, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219018"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/22205442","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=245640","label":"url"}],"paper_title":{"en":"Enhancement of sialylation on humanized lgG-like bispecific antibody by overexpression of 2,6-sialyltransferase derived from Chainese hamster ovary cells","ja":"Enhancement of sialylation on humanized lgG-like bispecific antibody by overexpression of 2,6-sialyltransferase derived from Chainese hamster ovary cells"},"authors":{"en":[{"name":"Onitsuka Masayoshi"},{"name":"Kim Wook-Dong"},{"name":"Ozaki H."},{"name":"Kawaguchi Akira"},{"name":"Honda Kohsuke"},{"name":"Kajiura H."},{"name":"Fujiyama K."},{"name":"Asano Ryutaro"},{"name":"Kumagai Izumi"},{"name":"Ohtake Hisao"},{"name":"Omasa Takeshi"}],"ja":[{"name":"鬼塚 正義"},{"name":"Kim Wook-Dong"},{"name":"Ozaki H."},{"name":"Kawaguchi Akira"},{"name":"Honda Kohsuke"},{"name":"Kajiura H."},{"name":"Fujiyama K."},{"name":"Asano Ryutaro"},{"name":"Kumagai Izumi"},{"name":"Ohtake Hisao"},{"name":"大政 健史"}]},"description":{"en":"Improvement of glycosylation is one of the most important topics in the industrial production of therapeutic antibodies. We have focused on terminal sialylation with alpha-2,6 linkage, which is crucial for anti-inflammatory activity. In the present study, we have successfully cloned cDNA of beta-galactosyl alpha-2,6 sialyltransferase (ST6Gal I) derived from Chinese hamster ovary (CHO) cells regardless of reports that stated this was not endogenously expressed in CHO cells. After expressing cloned ST6Gal I in Escherichia coli, the transferase activity was confirmed by HPLC and lectin binding assay. Then, we applied ST6Gal I to alpha-2,6 sialylation of the recombinant antibody; the ST6Gal I expression vector was transfected into the CHO cell line producing a bispecific antibody. The N-glycosylation pattern of the antibody was estimated by HPLC and sialidase digestion. About 70% of the total N-linked oligosaccharide was alpha-2,6 sialylated in the transfected cell line whereas no sialylation was observed in the non-transfected cell line. The improvement of sialylation would be of practical importance for the industrial production of therapeutic antibodies.","ja":"Improvement of glycosylation is one of the most important topics in the industrial production of therapeutic antibodies. We have focused on terminal sialylation with alpha-2,6 linkage, which is crucial for anti-inflammatory activity. In the present study, we have successfully cloned cDNA of beta-galactosyl alpha-2,6 sialyltransferase (ST6Gal I) derived from Chinese hamster ovary (CHO) cells regardless of reports that stated this was not endogenously expressed in CHO cells. After expressing cloned ST6Gal I in Escherichia coli, the transferase activity was confirmed by HPLC and lectin binding assay. Then, we applied ST6Gal I to alpha-2,6 sialylation of the recombinant antibody; the ST6Gal I expression vector was transfected into the CHO cell line producing a bispecific antibody. The N-glycosylation pattern of the antibody was estimated by HPLC and sialidase digestion. About 70% of the total N-linked oligosaccharide was alpha-2,6 sialylated in the transfected cell line whereas no sialylation was observed in the non-transfected cell line. The improvement of sialylation would be of practical importance for the industrial production of therapeutic antibodies."},"publication_date":"2012-04","publication_name":{"en":"Applied Microbiology and Biotechnology","ja":"Applied Microbiology and Biotechnology"},"volume":"Vol.94","number":"No.1","starting_page":"69","ending_page":"80","languages":["eng"],"referee":true,"identifiers":{"doi":["10.1007/s00253-011-3814-1"],"issn":["1432-0614"]},"published_paper_type":"scientific_journal"},"priority":"input_data"} line:26, {"insert":{"user_id":"R000014847","type":"published_papers","id":"31219019"},"force":{"see_also":[{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=315656","label":"url"}],"paper_title":{"en":"Increased antibody productivity in Chinese Hamster Ovary cells through induction of chromosomal instability by cell fusion","ja":"Increased antibody productivity in Chinese Hamster Ovary cells through induction of chromosomal instability by cell 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line"},"authors":{"en":[{"name":"Yamano Noriko"},{"name":"Kumamoto Toshitaka"},{"name":"Takahashi Mai"},{"name":"Frank Jana"},{"name":"Onitsuka Masayoshi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"山野 範子"},{"name":"Kumamoto Toshitaka"},{"name":"Takahashi Mai"},{"name":"フランク ヤナ"},{"name":"鬼塚 正義"},{"name":"大政 健史"}]},"publication_date":"2015-12","publication_name":{"en":"BMC Proceedings","ja":"BMC Proceedings"},"volume":"Vol.9","number":"No.Supplement 9","starting_page":"P1","ending_page":"P1","languages":["eng"],"identifiers":{"doi":["10.1186/1753-6561-9-S9-P1"],"issn":["1753-6561"]},"published_paper_type":"research_institution"},"priority":"input_data"} ==== end registerFile(/WWW/pub2/data/ERD/person/246724/researchmap/published_papers.jsonl, ZsEw-I4B7kacV6CWePxK) ==== ==== begin registerFile(/WWW/pub2/data/ERD/person/246724/researchmap/misc.jsonl) ==== line:1, 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{"insert":{"user_id":"R000014847","type":"misc","id":"31219025"},"force":{"see_also":[{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=219583","label":"url"}],"paper_title":{"en":"生産細胞の品質保証について考える-はたしてゲノム解析はパンドラの匣か-","ja":"生産細胞の品質保証について考える-はたしてゲノム解析はパンドラの匣か-"},"authors":{"en":[{"name":"曹 溢華"},{"name":"木村 修一"},{"name":"Onitsuka Masayoshi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"曹 溢華"},{"name":"木村 修一"},{"name":"鬼塚 正義"},{"name":"大政 健史"}]},"publication_date":"2010-12","publication_name":{"en":"PHARM TECH JAPAN","ja":"ファームテクジャパン"},"volume":"Vol.26","number":"No.13","starting_page":"95","ending_page":"102","languages":["jpn"],"misc_type":"introduction_scientific_journal"},"priority":"input_data"} line:4, {"insert":{"user_id":"R000014847","type":"misc","id":"31219026"},"force":{"see_also":[{"@id":"https://www.ncbi.nlm.nih.gov/pubmed/20210750","label":"url"},{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=208863","label":"url"}],"paper_title":{"en":"Cell engineering and cultivation of Chinese hamster ovary (CHO) cells","ja":"Cell engineering and cultivation of Chinese hamster ovary (CHO) cells"},"authors":{"en":[{"name":"Omasa Takeshi"},{"name":"Onitsuka Masayoshi"},{"name":"Kim Wook-Dong"}],"ja":[{"name":"大政 健史"},{"name":"鬼塚 正義"},{"name":"Kim Wook-Dong"}]},"description":{"en":"Mammalian cell lines are important host cells for the industrial production of pharmaceutical proteins owing to their capacity for correct folding, assembly and post-translational modification. In particular, Chinese hamster ovary (CHO) cells are the most dependable host cells for the industrial production of therapeutic proteins. Growing demand for therapeutic proteins promotes the development of technologies for high quality and productivity in CHO expression systems. The following are fundamentally important for effective production. 1) Construction of cultivation process. The CHO-based cultivation process is well established and is a general platform of therapeutic antibody production. The cost of therapeutic protein production using CHO cells is equivalent to that using microbial culture. 2) Cell line development. Recent developments in omics technologies have been essential for the development of rational methods of constructing a cell line. 3) Cell engineering for post-translational steps. Improvement of secretion, folding and glycosylaiton is an important key issue for mammalian cell production systems. This review provides an overview of the industrial production of therapeutic proteins using a CHO cell expression system.","ja":"Mammalian cell lines are important host cells for the industrial production of pharmaceutical proteins owing to their capacity for correct folding, assembly and post-translational modification. In particular, Chinese hamster ovary (CHO) cells are the most dependable host cells for the industrial production of therapeutic proteins. Growing demand for therapeutic proteins promotes the development of technologies for high quality and productivity in CHO expression systems. The following are fundamentally important for effective production. 1) Construction of cultivation process. The CHO-based cultivation process is well established and is a general platform of therapeutic antibody production. The cost of therapeutic protein production using CHO cells is equivalent to that using microbial culture. 2) Cell line development. Recent developments in omics technologies have been essential for the development of rational methods of constructing a cell line. 3) Cell engineering for post-translational steps. Improvement of secretion, folding and glycosylaiton is an important key issue for mammalian cell production systems. This review provides an overview of the industrial production of therapeutic proteins using a CHO cell expression system."},"publication_date":"2010-04","publication_name":{"en":"Current Pharmaceutical Biotechnology","ja":"Current Pharmaceutical Biotechnology"},"volume":"Vol.11","number":"No.3","starting_page":"232","ending_page":"240","languages":["eng"],"identifiers":{"doi":["10.2174/138920110791111960"],"issn":["1873-4316"]},"misc_type":"introduction_scientific_journal"},"priority":"input_data"} ==== end registerFile(/WWW/pub2/data/ERD/person/246724/researchmap/misc.jsonl, asEw-I4B7kacV6CWefwD) ==== ==== begin registerFile(/WWW/pub2/data/ERD/person/246724/researchmap/books_etc.jsonl) ==== line:1, 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正義"}]},"publisher":{"en":"サイエンス&テクノロジー","ja":"サイエンス&テクノロジー"},"publication_date":"2022-10-26","languages":["jpn"]},"priority":"input_data"} line:3, {"insert":{"user_id":"R000014847","type":"books_etc","id":"39666213"},"force":{"see_also":[{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=390168","label":"url"}],"book_title":{"en":"抗体生産CHO細胞の培養プロセスにおける凝集化抗体の発生化機構と抑制への考察","ja":"抗体生産CHO細胞の培養プロセスにおける凝集化抗体の発生化機構と抑制への考察"},"authors":{"en":[{"name":"Onitsuka Masayoshi"}],"ja":[{"name":"鬼塚 正義"}]},"publisher":{"en":"Technical Information Institute Co., Ltd.","ja":"株式会社 技術情報協会"},"publication_date":"2021-04-30","languages":["jpn"]},"priority":"input_data"} line:4, {"insert":{"user_id":"R000014847","type":"books_etc","id":"31219040"},"force":{"see_also":[{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=356933","label":"url"}],"book_title":{"en":"培養プロセスにおける凝集形成と制御について ∼抗体生産CHO細胞を中心に∼","ja":"培養プロセスにおける凝集形成と制御について ∼抗体生産CHO細胞を中心に∼"},"authors":{"en":[{"name":"Onitsuka Masayoshi"}],"ja":[{"name":"鬼塚 正義"}]},"publisher":{"en":"サイエンス&テクノロジー","ja":"サイエンス&テクノロジー"},"publication_date":"2019-08-27","languages":["jpn"]},"priority":"input_data"} line:5, {"insert":{"user_id":"R000014847","type":"books_etc","id":"31219041"},"force":{"see_also":[{"@id":"https://web.db.tokushima-u.ac.jp/cgi-bin/edb_browse?EID=311848","label":"url"}],"book_title":{"en":"第3編 細胞構築・培地設計 第4章ケミカルシャペロンを用いた蛋白質凝集防止培地の開発","ja":"第3編 細胞構築・培地設計 第4章ケミカルシャペロンを用いた蛋白質凝集防止培地の開発"},"authors":{"en":[{"name":"Onitsuka Masayoshi"},{"name":"Omasa Takeshi"}],"ja":[{"name":"鬼塚 正義"},{"name":"大政 健史"}]},"publisher":{"en":"株式会社シーエムシー出版","ja":"株式会社シーエムシー出版"},"publication_date":"2015-03","languages":["jpn"]},"priority":"input_data"} line:6, 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