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Dive into the research topics where Kouichi Shiosaki is active.

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Featured researches published by Kouichi Shiosaki.


Journal of Virology | 2006

Sequential Immunization with V3 Peptides from Primary Human Immunodeficiency Virus Type 1 Produces Cross-Neutralizing Antibodies against Primary Isolates with a Matching Narrow-Neutralization Sequence Motif

Yasuyuki Eda; Mari Takizawa; Toshio Murakami; Hiroaki Maeda; Kazuhiko Kimachi; Hiroshi Yonemura; Satoshi Koyanagi; Kouichi Shiosaki; Hirofumi Higuchi; Keiichi Makizumi; Toshihiro Nakashima; Kiyoshi Osatomi; Sachio Tokiyoshi; Shuzo Matsushita; Naoki Yamamoto; Mitsuo Honda

ABSTRACT An antibody response capable of neutralizing not only homologous but also heterologous forms of the CXCR4-tropic human immunodeficiency virus type 1 (HIV-1) MNp and CCR5-tropic primary isolate HIV-1 JR-CSF was achieved through sequential immunization with a combination of synthetic peptides representing HIV-1 Env V3 sequences from field and laboratory HIV-1 clade B isolates. In contrast, repeated immunization with a single V3 peptide generated antibodies that neutralized only type-specific laboratory-adapted homologous viruses. To determine whether the cross-neutralization response could be attributed to a cross-reactive antibody in the immunized animals, we isolated a monoclonal antibody, C25, which neutralized the heterologous primary viruses of HIV-1 clade B. Furthermore, we generated a humanized monoclonal antibody, KD-247, by transferring the genes of the complementary determining region of C25 into genes of the human V region of the antibody. KD-247 bound with high affinity to the “PGR” motif within the HIV-1 Env V3 tip region, and, among the established reference antibodies, it most effectively neutralized primary HIV-1 field isolates possessing the matching neutralization sequence motif, suggesting its promise for clinical applications involving passive immunizations. These results demonstrate that sequential immunization with B-cell epitope peptides may contribute to a humoral immune-based HIV vaccine strategy. Indeed, they help lay the groundwork for the development of HIV-1 vaccine strategies that use sequential immunization with biologically relevant peptides to overcome difficulties associated with otherwise poorly immunogenic epitopes.


Pharmaceutical Research | 1998

Microencapsulation of Hepatitis B Core Antigen for Vaccine Preparation

Takahiro Uchida; Kouichi Shiosaki; Yoichi Nakada; Katsuhiko Fukada; Yasuyuki Eda; Sachio Tokiyoshi; Noriko Nagareya; Kenji Matsuyama

AbstractPurpose. To prepare poly(lactide-co-glycolide)(PLGA) microspheres containing recombinant hepatitis B core antigen (HBcAg; Mw = 3,600,000) by a w/o/w emulsion/solvent evaporation method and evaluate the possibility of this system as a potent long-acting carrier for hepatitis B core antigen in mice. Methods. Various additives had been incorporated in the internal aqueous phase during the process of microencapsulating HBcAg, HBcAg antigenicity in the medium extracted from the prepared microspheres were measured by ELISA. Shape confirmation of the HBcAg antigen was performed by a sucrose gradient velocity centrifugal technique. For in vivo study, prepared microspheres were administered subcutaneously to Balb/C mice, and the serum IgG level was determined by ELISA. Results. The inactivation of HBcAg by methylene chloride was dramatically reduced by the addition of gelatin (4−8% (w/v)) to the internal aqueous phase during the preparation. Further improvement of the loading efficiency to almost 61% resulted with cooling (4°C). The prepared microspheres (4.27 μm ± 1.23 μm) containing 0.15% HBcAg displayed burst release (50−60% within 2 days). In subcutaneous inoculation, the adjuvant effect of PLGA microspheres was almost the same as that of the complete Freunds adjuvant. Whereas oral inoculation using the microspheres was not effective. Conclusions. The pH of the added gelatin seemed to be the key to the stabilization of HBcAg from various stability tests and CD spectrum study. Finally, the possibility of using this system as a potent long-acting hepatitis B vaccine was demonostrated.


Archive | 1994

Anti-hiv monoclonal antibody

Yasuyuki Eda; Hiroaki Maeda; Keiichi Makizumi; Kouichi Shiosaki; Kiyoshi Osatomi; Kazuhiko Kimachi; Hirofumi Higuchi; Sachio Tokiyoshi


Archive | 1993

Recombinant anti-HIV antibody and process for preparing the same

Hiroaki Maeda; Kazuhiko Kimachi; Yasuyuki Eda; Kouichi Shiosaki; Kiyoshi Osatomi; Sachio Tokiyoshi


Clinical Immunology | 2004

Hemagglutinating virus of Japan protein is efficient for induction of CD4+ T-cell response by a hepatitis B core particle-based HIV vaccine.

Satoshi Takeda; Kouichi Shiosaki; Yasufumi Kaneda; Hitomi Yoshizaki; Kenji Someya; Yusuke Konno; Yasuyuki Eda; Youichirou Kino; Naoki Yamamoto; Mitsuo Honda


Archive | 1992

Human immunodeficiency virus-related immune preparation

Yasuyuki Eda; Kouichi Shiosaki; Kiyoshi Osatomi; Sachio Tokiyoshi


Archive | 1994

HIV monoclonal antibody specific for the HTLV-IIImn gp120 envelope glycoprotein

Yasuyuki Eda; Kiyoshi Osatomi; Kouichi Shiosaki; Sachio Tokiyoshi; Shuzo Matsushita; Toshio Hattori; Kiyoshi Takatsuki


Archive | 1991

Anti HTLV-III (strain MN) monoclonal antibody

Yasuyuki Eda; Kiyoshi Osatomi; Kouichi Shiosaki; Sachio Tokiyoshi; Shuzo Matsushita; Toshio Hattori; Kiyoshi Takatsuki


Archive | 1993

Recombinant anti-hiv antibody and preparation thereof

Hiroaki Maeda; Kazuhiko Kimachi; Yasuyuki Eda; Kouichi Shiosaki; Kiyoshi Osatomi; Sachio Tokiyoshi


Archive | 1995

PRODUCTION OF PROTEIN SUSTAINED RELEASE MICROSPHERE

Katsuhiko Fukada; Yoichi Nakada; Kouichi Shiosaki; Yukio Tokiyoshi; Takahiro Uchida; 洋一 中田; 享弘 内田; 巧一 塩先; 幸男 時吉; 勝彦 深田

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Yasuyuki Eda

Medical Research Council

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Hirofumi Higuchi

Sumitomo Electric Industries

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Takahiro Uchida

Mukogawa Women's University

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Yoichi Nakada

Mukogawa Women's University

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