Your search keyword '"Kazuyoshi Ikuta"' showing total 460 results

1. Chimeric flavivirus enables evaluation of antibodies against dengue virus envelope protein in vitro and in vivo

Author

Takeshi Kurosu, Keiko Hanabara, Azusa Asai, Sabar Pambudi, Supranee Phanthanawiboon, Magot Diata Omokoko, Ken-ichiro Ono, Masayuki Saijo, Pongrama Ramasoota, and Kazuyoshi Ikuta

Subjects

Medicine, Science

Abstract

Abstract In a secondary dengue virus (DENV) infection, the presence of non-neutralizing antibodies (Abs), developed during a previous infection with a different DENV serotype, is thought to worsen clinical outcomes by enhancing viral production. This phenomenon is called antibody-dependent enhancement (ADE) of infection, and it has delayed the development of therapeutic Abs and vaccines against DENV, as they must be evaluated for the potential to induce ADE. Unfortunately, limited replication of DENV clinical isolates in vitro and in experimental animals hinders this evaluation process. We have, therefore, constructed a recombinant chimeric flavivirus (DV2ChimV), which carries premembrane (prM) and envelope (E) genes of type 2 DENV (DENV-2) R05-624 clinical (Thai) isolate in a backbone of Japanese encephalitis virus (Nakayama strain). DENV E-protein is the most important viral target, not only for neutralizing Abs, but also for infection-enhancing Abs. In contrast to DENV-2 R05-624, DV2ChimV replicated efficiently in cultured mammalian cells and was lethal in interferon-α/β–γ-receptor double-knockout mice. With DV2ChimV, we were able to perform neutralization assays, in vitro and in vivo ADE assays, and in vivo protection assays. These results suggest that the chimeric virus is a powerful tool for evaluation of Abs against DENV.

Published

2020

2. Ongoing rubella epidemic in Osaka, Japan in 2018–2019

Author

Daiki Kanbayashi, Takako Kurata, Hideyuki Kubo, Atsushi Kaida, Seiji P Yamamoto, Kazutaka Egawa, Yuki Hirai, Kazuma Okada, Ryo Ikemori, Takahiro Yumisashi, Akira Yamamoto, Hideki Yoshida, Takanori Hirayama, Kazuyoshi Ikuta, and Kazushi Motomura

Subjects

rubella, rubella virus, japan, genotype 1e, viruses, Medicine, Public aspects of medicine, RA1-1270

Abstract

A large rubella epidemic is currently ongoing since 2018 in Osaka, Japan. The detected rubella viruses were classified into genotypes 1E lineage 2 and 2B lineage 1. These strains may have been imported from endemic countries, and these viruses spread within the susceptible population.

Published

2021

3. A Broadly Reactive Human Anti-hemagglutinin Stem Monoclonal Antibody That Inhibits Influenza A Virus Particle Release

Author

Seiya Yamayoshi, Ryuta Uraki, Mutsumi Ito, Maki Kiso, Sumiho Nakatsu, Atsuhiro Yasuhara, Kohei Oishi, Tadahiro Sasaki, Kazuyoshi Ikuta, and Yoshihiro Kawaoka

Subjects

Influenza A virus, Human monoclonal antibody, HA stem, Broadly reactive, Medicine, Medicine (General), R5-920

Abstract

Many broadly reactive human monoclonal antibodies against the hemagglutinin (HA) stem of influenza A virus have been developed for therapeutic applications. These antibodies typically inhibit viral entry steps, especially the HA conformational change that is required for membrane fusion. To better understand the mechanisms by which such antibodies inhibit viral replication, we established broadly reactive human anti-HA stem antibodies and determined the properties of these antibodies by examining their reactivity with 18 subtypes of HA, evaluating their in vivo protective efficacy, identifying their epitopes, and characterizing their inhibitory mechanisms. Among the eight human monoclonal antibodies we generated, which recognized at least 3 subtypes of the soluble HA antigens tested, clone S9-1-10/5-1 reacted with 18 subtypes of HA and protected mice from lethal infection with H1N1pdm09, H3N2, H5N1, and H7N9 viruses. This antibody recognized the HA2 helix A in the HA stem, and inhibited virus particle release from infected cells but did not block viral entry completely. These results show that broadly reactive human anti-HA stem antibodies can exhibit protective efficacy by inhibiting virus particle release. These findings expand our knowledge of the mechanisms by which broadly reactive stem-targeting antibodies inhibit viral replication and provide valuable information for universal vaccine development.

Published

2017

4. Two Different Strains of Severe Fever with Thrombocytopenia Syndrome Virus (SFTSV) in North and South Osaka by Phylogenetic Analysis of Evolutionary Lineage: Evidence for Independent SFTSV Transmission

Author

Ryo Ikemori, Ikuko Aoyama, Tadahiro Sasaki, Hirono Takabayashi, Kazutoshi Morisada, Masaru Kinoshita, Kazuyoshi Ikuta, Takahiro Yumisashi, and Kazushi Motomura

Subjects

SFTS, genotype, whole genome, Microbiology, QR1-502

Abstract

Severe fever with thrombocytopenia syndrome (SFTS) is a novel tick-borne infectious disease, therefore, the information on the whole genome of the SFTS virus (SFTSV) is still limited. This study demonstrates a nearly whole genome of the SFTSV identified in Osaka in 2017 and 2018 by next-generation sequencing (NGS). The evolutionary lineage of two genotypes, C5 and J1, was identified in Osaka. The first case in Osaka belongs to suspect reassortment (L:C5, M:C5, S:C4), the other is genotype J1 (L: J1, M: J1, S: J1) according to the classification by a Japanese group. C5 was identified in China, indicating that C5 identified in this study may be transmitted by birds between China and Japan. This study revealed that different SFTSV genotypes were distributed in two local areas, suggesting the separate or focal transmission patterns in Osaka.

Published

2021

5. Fully Human Monoclonal Antibodies Effectively Neutralizing Botulinum Neurotoxin Serotype B

Author

Takuhiro Matsumura, Sho Amatsu, Ryo Misaki, Masahiro Yutani, Anariwa Du, Tomoko Kohda, Kazuhito Fujiyama, Kazuyoshi Ikuta, and Yukako Fujinaga

Subjects

Clostridium botulinum, neurotoxin, botulism, fully human monoclonal antibody, SPYMEG, therapeutic effect, Medicine

Abstract

Botulinum neurotoxin (BoNT) is the most potent natural toxin known. Of the seven BoNT serotypes (A to G), types A, B, E, and F cause human botulism. Treatment of human botulism requires the development of effective toxin-neutralizing antibodies without side effects such as serum sickness and anaphylaxis. In this study, we generated fully human monoclonal antibodies (HuMAbs) against serotype B BoNT (BoNT/B1) using a murine–human chimera fusion partner cell line named SPYMEG. Of these HuMAbs, M2, which specifically binds to the light chain of BoNT/B1, showed neutralization activity in a mouse bioassay (approximately 10 i.p. LD50/100 µg of antibody), and M4, which binds to the C-terminal of heavy chain, showed partial protection. The combination of two HuMAbs, M2 (1.25 µg) and M4 (1.25 µg), was able to completely neutralize BoNT/B1 (80 i.p. LD50) with a potency greater than 80 i.p. LD50/2.5 µg of antibodies, and was effective both prophylactically and therapeutically in the mouse model of botulism. Moreover, this combination showed broad neutralization activity against three type B subtypes, namely BoNT/B1, BoNT/B2, and BoNT/B6. These data demonstrate that the combination of M2 and M4 is promising in terms of a foundation for new human therapeutics for BoNT/B intoxication.

Published

2020

6. Novel Polymerase Gene Mutations for Human Adaptation in Clinical Isolates of Avian H5N1 Influenza Viruses.

Author

Yasuha Arai, Norihito Kawashita, Tomo Daidoji, Madiha S Ibrahim, Emad M El-Gendy, Tatsuya Takagi, Kazuo Takahashi, Yasuo Suzuki, Kazuyoshi Ikuta, Takaaki Nakaya, Tatsuo Shioda, and Yohei Watanabe

Subjects

Immunologic diseases. Allergy, RC581-607, Biology (General), QH301-705.5

Abstract

A major determinant in the change of the avian influenza virus host range to humans is the E627K substitution in the PB2 polymerase protein. However, the polymerase activity of avian influenza viruses with a single PB2-E627K mutation is still lower than that of seasonal human influenza viruses, implying that avian viruses require polymerase mutations in addition to PB2-627K for human adaptation. Here, we used a database search of H5N1 clade 2.2.1 virus sequences with the PB2-627K mutation to identify other polymerase adaptation mutations that have been selected in infected patients. Several of the mutations identified acted cooperatively with PB2-627K to increase viral growth in human airway epithelial cells and mouse lungs. These mutations were in multiple domains of the polymerase complex other than the PB2-627 domain, highlighting a complicated avian-to-human adaptation pathway of avian influenza viruses. Thus, H5N1 viruses could rapidly acquire multiple polymerase mutations that function cooperatively with PB2-627K in infected patients for optimal human adaptation.

Published

2016

7. Characterization of H5N1 Influenza Virus Variants with Hemagglutinin Mutations Isolated from Patients

Author

Yohei Watanabe, Yasuha Arai, Tomo Daidoji, Norihito Kawashita, Madiha S. Ibrahim, Emad El-Din M. El-Gendy, Hiroaki Hiramatsu, Ritsuko Kubota-Koketsu, Tatsuya Takagi, Takeomi Murata, Kazuo Takahashi, Yoshinobu Okuno, Takaaki Nakaya, Yasuo Suzuki, and Kazuyoshi Ikuta

Subjects

Microbiology, QR1-502

Abstract

ABSTRACT A change in viral hemagglutinin (HA) receptor binding specificity from α2,3- to α2,6-linked sialic acid is necessary for highly pathogenic avian influenza (AI) virus subtype H5N1 to become pandemic. However, details of the human-adaptive change in the H5N1 virus remain unknown. Our database search of H5N1 clade 2.2.1 viruses circulating in Egypt identified multiple HA mutations that had been selected in infected patients. Using reverse genetics, we found that increases in both human receptor specificity and the HA pH threshold for membrane fusion were necessary to facilitate replication of the virus variants in human airway epithelia. Furthermore, variants with enhanced replication in human cells had decreased HA stability, apparently to compensate for the changes in viral receptor specificity and membrane fusion activity. Our findings showed that H5N1 viruses could rapidly adapt to growth in the human airway microenvironment by altering their HA properties in infected patients and provided new insights into the human-adaptive mechanisms of AI viruses. IMPORTANCE Circulation between bird and human hosts may allow H5N1 viruses to acquire amino acid changes that increase fitness for human infections. However, human-adaptive changes in H5N1 viruses have not been adequately investigated. In this study, we found that multiple HA mutations were actually selected in H5N1-infected patients and that H5N1 variants with some of these HA mutations had increased human-type receptor specificity and increased HA membrane fusion activity, both of which are advantageous for viral replication in human airway epithelia. Furthermore, HA mutants selected during viral replication in patients were likely to have less HA stability, apparently as a compensatory mechanism. These results begin to clarify the picture of the H5N1 human-adaptive mechanism.

Published

2015

8. Molecular characterization of Clostridium botulinum isolates from foodborne outbreaks in Thailand, 2010.

Author

Piyada Wangroongsarb, Tomoko Kohda, Chutima Jittaprasartsin, Karun Suthivarakom, Thanitchi Kamthalang, Kaoru Umeda, Pathom Sawanpanyalert, Shunji Kozaki, and Kazuyoshi Ikuta

Subjects

Medicine, Science

Abstract

BACKGROUND: Thailand has had several foodborne outbreaks of botulism, one of the biggest being in 2006 when laboratory investigations identified the etiologic agent as Clostridium botulinum type A. Identification of the etiologic agent from outbreak samples is laborious using conventional microbiological methods and the neurotoxin mouse bioassay. Advances in molecular techniques have added enormous information regarding the etiology of outbreaks and characterization of isolates. We applied these methods in three outbreaks of botulism in Thailand in 2010. METHODOLOGY/PRINCIPAL FINDINGS: A total of 19 cases were involved (seven each in Lampang and Saraburi and five in Maehongson provinces). The first outbreak in Lampang province in April 2010 was associated with C. botulinum type F, which was detected by conventional methods. Outbreaks in Saraburi and Maehongson provinces occurred in May and December were due to C. botulinum type A1(B) and B that were identified by conventional methods and molecular techniques, respectively. The result of phylogenetic sequence analysis showed that C. botulinum type A1(B) strain Saraburi 2010 was close to strain Iwate 2007. Molecular analysis of the third outbreak in Maehongson province showed C. botulinum type B8, which was different from B1-B7 subtype. The nontoxic component genes of strain Maehongson 2010 revealed that ha33, ha17 and botR genes were close to strain Okra (B1) while ha70 and ntnh genes were close to strain 111 (B2). CONCLUSION/SIGNIFICANCE: This study demonstrates the utility of molecular genotyping of C. botulinum and how it contributes to our understanding the epidemiology and variation of boNT gene. Thus, the recent botulism outbreaks in Thailand were induced by various C. botulinum types.

Published

2014

9. Low levels of antibody-dependent enhancement in vitro using viruses and plasma from dengue patients.

Author

Panjaporn Chaichana, Tamaki Okabayashi, Orapim Puiprom, Mikiko Sasayama, Tadahiro Sasaki, Akifumi Yamashita, Pongrama Ramasoota, Takeshi Kurosu, and Kazuyoshi Ikuta

Subjects

Medicine, Science

Abstract

BACKGROUND: The majority of dengue patients infected with any serotype of dengue virus (DENV) are asymptomatic, but the remainder may develop a wide spectrum of clinical symptoms, ranging from mild dengue fever (DF) to severe dengue hemorrhagic fever (DHF). Severe cases occur more often in patients who experience a secondary infection with a different virus serotype. A phenomenon called antibody-dependent enhancement (ADE) has been proposed to explain the onset of these severe cases, but the exact mechanism of ADE remains unclear. METHODOLOGY/PRINCIPAL FINDING: Virus neutralization and ADE assays were performed using ultracentrifugation supernatants of acute-phase sera from patients with secondary infections or human monoclonal antibodies (HuMAbs) as anti-DENV antibodies. Virus sources included infectious serum-derived viruses from the ultracentrifugation precipitates, laboratory-culture adapted DENV, or recombinant DENVs derived from patient sera. In contrast to the high levels of ADE observed with laboratory virus strains, low ADE was observed with autologous patient-derived viruses, when patient sera were used to provide the antibody component in the ADE assays. Similar results were obtained using samples from DF and DHF patients. Recombinant-viruses derived from DHF patients showed only minor differences in neutralization and ADE activity in the presence of HuMAbs or plasma derived from the same DHF patient. CONCLUSION/SIGNIFICANCE: Serum or plasma taken from patients during the acute phase of a secondary infection showed high levels of ADE, but no neutralization activity, when assayed in the presence of laboratory-adapted virus strains. By contrast, serum or plasma from the same patient showed high levels of neutralization activity but failed to induce significant ADE when the assays were performed with autologous virus. These results demonstrate the significance of the virus source when measuring ADE. They also suggest that repeated passage of DENV in cell culture has endowed it with the capacity to induce high levels of ADE.

Published

2014

10. Isolation of Neutralizing Antibody

Author

Mayo Yasugi and Kazuyoshi Ikuta

Subjects

Biology (General), QH301-705.5

Abstract

Use of monoclonal antibodies (MAbs) is an established laboratory strategy for characterization of specific pathogens and their antigenicity. Especially, Human MAbs (HuMAbs) with neutralizing activity against specific virus could have potential therapeutic application, and provide significant information on human epitopes that could be important for developing the next generation of universal vaccines against the virus. In addition to the classical method for murine MAb preparation, several methods for the preparation of HuMAbs have been developed. Here, we describe the development of neutralizing HuMAbs against specific virus. HuMAbs are established by fusion of the peripheral blood mononuclear cells of vaccinated volunteers or patients with the fusion partner cell line, named SPYMEG. Then each of prepared HuMAbs is confirmed whether it can neutralize the specific virus by in vitro neutralization assay.

Published

2013

11. Influenza Virus-cell Fusion Inhibition Assay

Author

Mayo Yasugi and Kazuyoshi Ikuta

Subjects

Biology (General), QH301-705.5

Abstract

During viral infection to host cells, several viruses undergo the process of endocytosis and pH-dependent fusion. By fusion of viral membrane with host cellular membrane, the viral core invades to host cytoplasm. A part of monoclonal antibodies against viral membrane protein have potential to inhibit the viral fusion step. Here we describe in vitro influenza virus-cell fusion inhibition assay. The infected cells expressing viral membrane protein, such as hemagglutinin (HA), on cellular surface are incubated with monoclonal antibodies targeting viral membrane protein. Then the cells are incubated under low pH condition. If the antibody does not inhibit the fusion step, we can see multinucleated giant cells.

Published

2013

12. Surface Plasmon Resonance Analysis of Antigen-Antibody Interaction

Author

Mitsuhiro Nishimura and Kazuyoshi Ikuta

Subjects

Biology (General), QH301-705.5

Abstract

Molecular interaction between monoclonal antibodies (MAbs) and their recognized antigen is a fundamental event leading to the neutralization activity. Estimation of their binding affinity gives beneficial information to characterize the MAbs and to develop more effective MAbs. Surface plasmon resonance (SPR) analysis is a powerful tool to analyze the molecular interaction, enabling rapid and repetitive estimation with relatively small amount of sample. Here we describe a general protocol about SPR analysis on the interaction between viral antigen and human MAb (HuMAb) IgG. Anti-human Fcγ is first covalently crosslinked on the sensor chip by amine coupling, and then HuMAb of interest is immobilized via anti-Fcγ MAb IgG interaction as ligand. Antigen injected on the sensor chip causes the SPR change in time course as the result of association and dissociation. By analyzing the kinetics, association rate, dissociation rate, and dissociation constant are obtained.

Published

2013

13. Human monoclonal antibodies broadly neutralizing against influenza B virus.

Author

Mayo Yasugi, Ritsuko Kubota-Koketsu, Akifumi Yamashita, Norihito Kawashita, Anariwa Du, Tadahiro Sasaki, Mitsuhiro Nishimura, Ryo Misaki, Motoki Kuhara, Naphatsawan Boonsathorn, Kazuhito Fujiyama, Yoshinobu Okuno, Takaaki Nakaya, and Kazuyoshi Ikuta

Subjects

Immunologic diseases. Allergy, RC581-607, Biology (General), QH301-705.5

Abstract

Influenza virus has the ability to evade host immune surveillance through rapid viral genetic drift and reassortment; therefore, it remains a continuous public health threat. The development of vaccines producing broadly reactive antibodies, as well as therapeutic strategies using human neutralizing monoclonal antibodies (HuMAbs) with global reactivity, has been gathering great interest recently. Here, three hybridoma clones producing HuMAbs against influenza B virus, designated 5A7, 3A2 and 10C4, were prepared using peripheral lymphocytes from vaccinated volunteers, and were investigated for broad cross-reactive neutralizing activity. Of these HuMAbs, 3A2 and 10C4, which recognize the readily mutable 190-helix region near the receptor binding site in the hemagglutinin (HA) protein, react only with the Yamagata lineage of influenza B virus. By contrast, HuMAb 5A7 broadly neutralizes influenza B strains that were isolated from 1985 to 2006, belonging to both Yamagata and Victoria lineages. Epitope mapping revealed that 5A7 recognizes 316G, 318C and 321W near the C terminal of HA1, a highly conserved region in influenza B virus. Indeed, no mutations in the amino acid residues of the epitope region were induced, even after the virus was passaged ten times in the presence of HuMAb 5A7. Moreover, 5A7 showed significant therapeutic efficacy in mice, even when it was administered 72 hours post-infection. These results indicate that 5A7 is a promising candidate for developing therapeutics, and provide insight for the development of a universal vaccine against influenza B virus.

Published

2013

14. Emerging antigenic variants at the antigenic site Sb in pandemic A(H1N1)2009 influenza virus in Japan detected by a human monoclonal antibody.

Author

Mayo Yasugi, Ritsuko Kubota-Koketsu, Akifumi Yamashita, Norihito Kawashita, Anariwa Du, Ryo Misaki, Motoki Kuhara, Naphatsawan Boonsathorn, Kazuhito Fujiyama, Yoshinobu Okuno, Takaaki Nakaya, and Kazuyoshi Ikuta

Subjects

Medicine, Science

Abstract

The swine-origin pandemic A(H1N1)2009 virus, A(H1N1)pdm09, is still circulating in parts of the human population. To monitor variants that may escape from vaccination specificity, antigenic characterization of circulating viruses is important. In this study, a hybridoma clone producing human monoclonal antibody against A(H1N1)pdm09, designated 5E4, was prepared using peripheral lymphocytes from a vaccinated volunteer. The 5E4 showed viral neutralization activity and inhibited hemagglutination. 5E4 escape mutants harbored amino acid substitutions (A189T and D190E) in the hemagglutinin (HA) protein, suggesting that 5E4 recognized the antigenic site Sb in the HA protein. To study the diversity of Sb in A(H1N1)pdm09, 58 viral isolates were obtained during the 2009/10 and 2010/11 winter seasons in Osaka, Japan. Hemagglutination-inhibition titers were significantly reduced against 5E4 in the 2010/11 compared with the 2009/10 samples. Viral neutralizing titers were also significantly decreased in the 2010/11 samples. By contrast, isolated samples reacted well to ferret anti-A(H1N1)pdm09 serum from both seasons. Nonsynonymous substitution rates revealed that the variant Sb and Ca2 sequences were being positively selected between 2009/10 and 2010/11. In 7,415 HA protein sequences derived from GenBank, variants in the antigenic sites Sa and Sb increased significantly worldwide from 2009 to 2013. These results indicate that the antigenic variants in Sb are likely to be in global circulation currently.

Published

2013

15. Reliability of a newly-developed immunochromatography diagnostic kit for pandemic influenza A/H1N1pdm virus: implications for drug administration.

Author

Tadahiro Sasaki, Ritsuko Kubota-Koketsu, Michihiro Takei, Tatsuo Hagihara, Shinichi Iwamoto, Takuya Murao, Kazuo Sawami, Daizou Fukae, Masahiro Nakamura, Eiichi Nagata, Akira Kawakami, Yuko Mitsubayashi, Masafumi Ohno, Yasuo Uehara, Takashi Fukukawa, Yuta Kanai, Mieko Kosaka, and Kazuyoshi Ikuta

Subjects

Medicine, Science

Abstract

BackgroundFor the diagnosis of seasonal influenza, clinicians rely on point-of-care testing (POCT) using commercially available kits developed against seasonal influenza viruses. However, POCT has not yet been established for the diagnosis of pandemic influenza A virus (H1N1pdm) infection due to the low sensitivity of the existing kits for H1N1pdm.Methodology/principal findingsAn immunochromatography (IC) test kit was developed based on a monoclonal antibody against H1N1pdm, which does not cross-react with seasonal influenza A or B viruses. The efficacy of this kit (PDM-IC kit) for the diagnosis of H1N1pdm infection was compared with that of an existing kit for the detection of seasonal influenza viruses (SEA-IC kit). Nasal swabs (n = 542) were obtained from patients with flu-like syndrome at 13 clinics in Osaka, Japan during the winter of 2010/2011. Among the 542 samples, randomly selected 332 were further evaluated for viral presence by reverse transcriptase polymerase chain reaction (RT-PCR). The PDM-IC kit versus the SEA-IC kit showed higher sensitivity to and specificity for H1N1pdm, despite several inconsistencies between the two kits or between the kits and RT-PCR. Consequently, greater numbers of false-negative and false-positive cases were documented when the SEA-IC kit was employed. Significant correlation coefficients for sensitivity, specificity, and negative prediction values between the two kits were observed at individual clinics, indicating that the results could be affected by clinic-related techniques for sampling and kit handling. Importantly, many patients (especially influenza-negative cases) were prescribed anti-influenza drugs that were incongruous with their condition, largely due to physician preference for patient responses to questionnaires and patient symptomology, as opposed to actual viral presence.Conclusions/significanceConcomitant use of SEA-IC and PDM-IC kits increased the likelihood of correct influenza diagnosis. Increasing the credibility of POCT is anticipated to decrease the inappropriate dispensing of anti-influenza drugs, thereby minimizing the emergence of drug-resistant H1N1pdm strains.

Published

2012

16. Frequency of D222G and Q223R hemagglutinin mutants of pandemic (H1N1) 2009 influenza virus in Japan between 2009 and 2010.

Author

Mayo Yasugi, Shota Nakamura, Tomo Daidoji, Norihito Kawashita, Ririn Ramadhany, Cheng-Song Yang, Teruo Yasunaga, Tetsuya Iida, Toshihiro Horii, Kazuyoshi Ikuta, Kazuo Takahashi, and Takaaki Nakaya

Subjects

Medicine, Science

Abstract

BACKGROUND: In April 2009, a novel swine-derived influenza A virus (H1N1pdm) emerged and rapidly spread around the world, including Japan. It has been suggested that the virus can bind to both 2,3- and 2,6-linked sialic acid receptors in infected mammals, in contrast to contemporary seasonal H1N1 viruses, which have a predilection for 2,6-linked sialic acid. METHODS/RESULTS: To elucidate the existence and transmissibility of α2,3 sialic acid-specific viruses in H1N1pdm, amino acid substitutions within viral hemagglutinin molecules were investigated, especially D187E, D222G, and Q223R, which are related to a shift from human to avian receptor specificity. Samples from individuals infected during the first and second waves of the outbreak in Japan were examined using a high-throughput sequencing approach. In May 2009, three specimens from mild cases showed D222G and/or Q223R substitutions in a minor subpopulation of viruses infecting these individuals. However, the substitutions almost disappeared in the samples from five mild cases in December 2010. The D187E substitution was not widespread in specimens, even in May 2009. CONCLUSIONS: These results suggest that α2,3 sialic acid-specific viruses, including G222 and R223, existed in humans as a minor population in the early phase of the pandemic, and that D222 and Q223 became more dominant through human-to-human transmission during the first and second waves of the epidemic. These results are consistent with the low substitution rates identified in seasonal H1N1 viruses in 2008.

Published

2012

17. Acquisition of human-type receptor binding specificity by new H5N1 influenza virus sublineages during their emergence in birds in Egypt.

Author

Yohei Watanabe, Madiha S Ibrahim, Hany F Ellakany, Norihito Kawashita, Rika Mizuike, Hiroaki Hiramatsu, Nogluk Sriwilaijaroen, Tatsuya Takagi, Yasuo Suzuki, and Kazuyoshi Ikuta

Subjects

Immunologic diseases. Allergy, RC581-607, Biology (General), QH301-705.5

Abstract

Highly pathogenic avian influenza A virus subtype H5N1 is currently widespread in Asia, Europe, and Africa, with 60% mortality in humans. In particular, since 2009 Egypt has unexpectedly had the highest number of human cases of H5N1 virus infection, with more than 50% of the cases worldwide, but the basis for this high incidence has not been elucidated. A change in receptor binding affinity of the viral hemagglutinin (HA) from α2,3- to α2,6-linked sialic acid (SA) is thought to be necessary for H5N1 virus to become pandemic. In this study, we conducted a phylogenetic analysis of H5N1 viruses isolated between 2006 and 2009 in Egypt. The phylogenetic results showed that recent human isolates clustered disproportionally into several new H5 sublineages suggesting that their HAs have changed their receptor specificity. Using reverse genetics, we found that these H5 sublineages have acquired an enhanced binding affinity for α2,6 SA in combination with residual affinity for α2,3 SA, and identified the amino acid mutations that produced this new receptor specificity. Recombinant H5N1 viruses with a single mutation at HA residue 192 or a double mutation at HA residues 129 and 151 had increased attachment to and infectivity in the human lower respiratory tract but not in the larynx. These findings correlated with enhanced virulence of the mutant viruses in mice. Interestingly, these H5 viruses, with increased affinity to α2,6 SA, emerged during viral diversification in bird populations and subsequently spread to humans. Our findings suggested that emergence of new H5 sublineages with α2,6 SA specificity caused a subsequent increase in human H5N1 influenza virus infections in Egypt, and provided data for understanding the virus's pandemic potential.

Published

2011

18. Molecular evolution of HIV-1 CRF01_AE Env in Thai patients.

Author

Samatchaya Boonchawalit, Duangrat Jullaksorn, Jiraporn Uttiyoung, Amara Yowang, Nongkran Krathong, Sununta Chautrakul, Akifumi Yamashita, Kazuyoshi Ikuta, Amornsak Roobsoong, Sangkom Kanitvittaya, Pathom Sawanpanyalert, and Masanori Kameoka

Subjects

Medicine, Science

Abstract

BACKGROUND: The envelope glycoproteins (Env), gp120 and gp41, are the most variable proteins of human immunodeficiency virus type 1 (HIV-1), and are the major targets of humoral immune responses against HIV-1. A circulating recombinant form of HIV-1, CRF01_AE, is prevalent throughout Southeast Asia; however, only limited information regarding the immunological characteristics of CRF01_AE Env is currently available. In this study, we attempted to examine the evolutionary pattern of CRF01_AE Env under the selection pressure of host immune responses. METHODOLOGY/PRINCIPAL FINDINGS: Peripheral blood samples were collected periodically over 3 years from 15 HIV-1-infected individuals residing in northern Thailand, and amplified env genes from the samples were subjected to computational analysis. The V5 region of gp120 showed highest variability in several samples over 3 years, whereas the V1/V2 and/or V4 regions of gp120 also showed high variability in many samples. In addition, the N-terminal part of the C3 region of gp120 showed highest amino acid diversity among the conserved regions of gp120. Chronological changes in the numbers of amino acid residues in gp120 variable regions and potential N-linked glycosylation (PNLG) sites are involved in increasing the variability of Env gp120. Furthermore, the C3 region contained several amino acid residues potentially under positive selection, and APOBEC3 family protein-mediated G to A mutations were frequently detected in such residues. CONCLUSIONS/SIGNIFICANCE: Several factors, including amino acid substitutions particularly in gp120 C3 and V5 regions as well as changes in the number of PNLG sites and in the length of gp120 variable regions, were revealed to be involved in the molecular evolution of CRF01_AE Env. In addition, a similar tendency was observed between CRF01_AE and subtype C Env with regard to the amino acid variation of gp120 V3 and C3 regions. These results may provide important information for understanding the immunological characteristics of CRF01_AE Env.

Published

2011

19. Autogenous translational regulation of the Borna disease virus negative control factor X from polycistronic mRNA using host RNA helicases.

Author

Yohei Watanabe, Naohiro Ohtaki, Yohei Hayashi, Kazuyoshi Ikuta, and Keizo Tomonaga

Subjects

Immunologic diseases. Allergy, RC581-607, Biology (General), QH301-705.5

Abstract

Borna disease virus (BDV) is a nonsegmented, negative-strand RNA virus that employs several unique strategies for gene expression. The shortest transcript of BDV, X/P mRNA, encodes at least three open reading frames (ORFs): upstream ORF (uORF), X, and P in the 5' to 3' direction. The X is a negative regulator of viral polymerase activity, while the P phosphoprotein is a necessary cofactor of the polymerase complex, suggesting that the translation of X is controlled rigorously, depending on viral replication. However, the translation mechanism used by the X/P polycistronic mRNA has not been determined in detail. Here we demonstrate that the X/P mRNA autogenously regulates the translation of X via interaction with host factors. Transient transfection of cDNA clones corresponding to the X/P mRNA revealed that the X ORF is translated predominantly by uORF-termination-coupled reinitiation, the efficiency of which is upregulated by expression of P. We found that P may enhance ribosomal reinitiation at the X ORF by inhibition of the interaction of the DEAD-box RNA helicase DDX21 with the 5' untranslated region of X/P mRNA, via interference with its phosphorylation. Our results not only demonstrate a unique translational control of viral regulatory protein, but also elucidate a previously unknown mechanism of regulation of polycistronic mRNA translation using RNA helicases.

Published

2009

20. Direct metagenomic detection of viral pathogens in nasal and fecal specimens using an unbiased high-throughput sequencing approach.

Author

Shota Nakamura, Cheng-Song Yang, Naomi Sakon, Mayo Ueda, Takahiro Tougan, Akifumi Yamashita, Naohisa Goto, Kazuo Takahashi, Teruo Yasunaga, Kazuyoshi Ikuta, Tetsuya Mizutani, Yoshiko Okamoto, Michihira Tagami, Ryoji Morita, Norihiro Maeda, Jun Kawai, Yoshihide Hayashizaki, Yoshiyuki Nagai, Toshihiro Horii, Tetsuya Iida, and Takaaki Nakaya

Subjects

Medicine, Science

Abstract

With the severe acute respiratory syndrome epidemic of 2003 and renewed attention on avian influenza viral pandemics, new surveillance systems are needed for the earlier detection of emerging infectious diseases. We applied a "next-generation" parallel sequencing platform for viral detection in nasopharyngeal and fecal samples collected during seasonal influenza virus (Flu) infections and norovirus outbreaks from 2005 to 2007 in Osaka, Japan. Random RT-PCR was performed to amplify RNA extracted from 0.1-0.25 ml of nasopharyngeal aspirates (N = 3) and fecal specimens (N = 5), and more than 10 microg of cDNA was synthesized. Unbiased high-throughput sequencing of these 8 samples yielded 15,298-32,335 (average 24,738) reads in a single 7.5 h run. In nasopharyngeal samples, although whole genome analysis was not available because the majority (>90%) of reads were host genome-derived, 20-460 Flu-reads were detected, which was sufficient for subtype identification. In fecal samples, bacteria and host cells were removed by centrifugation, resulting in gain of 484-15,260 reads of norovirus sequence (78-98% of the whole genome was covered), except for one specimen that was under-detectable by RT-PCR. These results suggest that our unbiased high-throughput sequencing approach is useful for directly detecting pathogenic viruses without advance genetic information. Although its cost and technological availability make it unlikely that this system will very soon be the diagnostic standard worldwide, this system could be useful for the earlier discovery of novel emerging viruses and bioterrorism, which are difficult to detect with conventional procedures.

Published

2009

21. Chimeric flavivirus causes vascular leakage and bone marrow suppression in a mouse model

Author

Takeshi Kurosu, Keiko Hanabara, Azusa Asai, Sabar Pambudi, Supranee Phanthanawiboon, Magot Diata Omokoko, Yusuke Sakai, Tadaki Suzuki, and Kazuyoshi Ikuta

Subjects

Biophysics, Cell Biology, Molecular Biology, Biochemistry

Published

2023

22. Effects of various disaccharide adaptations on recombinant IgA1 production in CHO-K1 suspension cells

Author

John Benson Dy Choa, Tadahiro Sasaki, Hiroyuki Kajiura, Kazuyoshi Ikuta, Kazuhito Fujiyama, and Ryo Misaki

Subjects

Clinical Biochemistry, Biomedical Engineering, Bioengineering, Cell Biology, Biotechnology

Abstract

Immunoglobulin A (IgA) has been showing potential as a new therapeutic antibody. However, recombinant IgA suffers from low yield. Supplementation of the medium is an effective approach to improving the production and quality of recombinant proteins. In this study, we adapted IgA1-producing CHO-K1 suspension cells to a high concentration (150 mM) of different disaccharides, namely sucrose, maltose, lactose, and trehalose, to improve the production and quality of recombinant IgA1. The disaccharide-adapted cell lines had slower cell growth rates, but their cell viability was extended compared to the nonadapted IgA1-producing cell line. Glucose consumption was exhausted in all cell lines except for the maltose-adapted one, which still contained glucose even after the 9th day of culturing. Lactate production was higher among the disaccharide-adapted cell lines. The specific productivity of the maltose-adapted IgA1-producing line was 4-fold that of the nonadapted line. In addition, this specific productivity was higher than in previous productions of recombinant IgA1 with a lambda chain. Lastly, secreted IgA1 aggregated in all cell lines, which may have been caused by self-aggregation. These results suggest that a high concentration of disaccharide-supplemented induced hyperosmolarity in the IgA1-producing CHO-K1 cell lines. In addition, the maltose-adapted CHO-K1 cell line benefited from having an additional source of carbohydrate.

Published

2023

23. Generation and therapeutic efficacy of the novel Fc-modified cross-neutralizing human monoclonal antibodies against dengue virus

Author

Subenya Injampa, Surachet Benjathummarak, Sujitra Keadsanti, Wilarat Puangmanee, Atsushi Yamanaka, Tadahiro Sasaki, Kazuyoshi Ikuta, Pongrama Ramasoota, and Pannamthip Pitaksajjakul

Abstract

Background Dengue disease is a mosquito-borne infection caused by four dengue virus serotypes (DENV1-4). Secondary infections can produce flavivirus cross-reactive antibodies at sub-neutralizing levels. This phenomenon can significantly increase the severity of secondary infections via antibody-dependent enhancement (ADE). ADE activity is associated with a high risk of viral infection in immune effector cells, triggering cytokine cascade and activating the complement system, which lead to severe symptoms. Despite extensive studies, therapeutic antibodies, particularly fully human monoclonal antibodies, which can be an option for immune passive therapy, have not yet been discovered. Methodology/Principal Findings This study generated LALA-mutated human monoclonal antibody clone B3B9 (LALA-B3B9 HuMAb) that can neutralize all four DENV serotypes without enhancing viral activity. The number of infected cells obtained with the ADE assay was compared among wild-type antibody (B3B9), and modified Fc, LALA-B3B9 HuMAb, and N297Q (N297Q-B3B9), with or without complement proteins. Moreover, the therapeutic efficacy of these HuMAbs against ADE infection by competing with natural antibodies in patients with acute dengue was determined using the in vitro suppression-of-enhancement assay in K562 cells. The novel Fc-modified antibody LALA-B3B9 (Leu234Ala/Leu235Ala mutations) could have a therapeutic effect. Further, it exhibited neutralization properties against all dengue virus serotypes without triggering ADE activity at any antibody concentration. This outcome was similar to that of the previous Fc-modified N297Q-B3B9 antibody (N297Q mutation). Moreover, the effect of complement protein on enhancing and neutralizing activities was evaluated to assess unwanted inflammatory responses to these therapeutic antibodies. Results showed that the elimination of complement activity could reduce the severity of dengue. The activities of LALA-B3B9 and N297Q-B3B9 HuMAbs were complement-independent in all dengue virus serotypes. Conclusions LALA-B3B9 and N297Q-B3B9 HuMAbs can prevent the suppression-of-enhancement activity in K562 cells caused by human DENV2. Hence, they are promising candidates for dengue treatment.

Published

2023

24. Virus Neutralization by Human Intravenous Immunoglobulin Against Influenza Virus Subtypes A/H5 and A/H7

Author

Ritsuko Kubota-Koketsu, Mikihiro Yunoki, Kazuyoshi Ikuta, and Yoshinobu Okuno

Subjects

0301 basic medicine, Virus Neutralization, avian influenza virus, 030204 cardiovascular system & hematology, medicine.disease_cause, Virus, 03 medical and health sciences, 0302 clinical medicine, Rheumatology, intravenous immunoglobulin, Pandemic, medicine, Immunology and Allergy, Targets and Therapy [Biologics], Pharmacology (medical), Original Research, chemistry.chemical_classification, Avian influenza virus, biology, business.industry, Gastroenterology, Virology, Influenza A virus subtype H5N1, Vaccination, neutralizing, 030104 developmental biology, Enzyme, Oncology, chemistry, A/H5, A/H7, biology.protein, Antibody, business

Abstract

Ritsuko Kubota-Koketsu,1,2,* Mikihiro Yunoki,3,* Yoshinobu Okuno,4 Kazuyoshi Ikuta1 1Department of Virology, Research Institute for Microbial Diseases, Osaka University, Osaka, Japan; 2Surveillance Section, Research and Production Technology Department, The Research Foundation for Microbial Diseases of Osaka University, Kagawa, Japan; 3Research and Development Division, Japan Blood Products Organization, Tokyo, Japan; 4Kanonji Institute, The Research Foundation for Microbial Diseases of Osaka University, Kagawa, Japan*These authors contributed equally to this workCorrespondence: Ritsuko Kubota-KoketsuDepartment of Viral Infections, Research Institute for Microbial Diseases, Osaka University, 3-1 Yamadaoka, Suita, Osaka, 565-0871, JapanTel +1-6-6879-8348Fax +1-6-6879-8347Email koketsu@biken.osaka-u.ac.jpMikihiro YunokiResearch and Development Division, Japan Blood Products Organization, 15F Tamachi Station Tower N, 3-1-1 Shibaura, Minato-ku, Tokyo, 108-0023, JapanTel +81-3-6435-6500Fax +81-3-6435-6274Email yunoki-mikihiro@jbpo.or.jpPurpose: Highly pathogenic avian influenza viruses are a threat to human health. Although donor populations have not experienced pandemic, they have been immunized by natural infections and/or vaccinations of influenza viruses such as A/H1N1, A/H3N2, and B. Therefore, it is considered that human intravenous immunoglobulin (IVIG) derived from healthy donors does not include IgG against avian influenza viruses. However, cross-reactivity has not been evaluated yet. In this study, cross-reactivity against the avian influenza virus A/H5N1, A/H7N1, A/H7N2, A/H7N7, A/H7N9, and A/H10N9 was evaluated.Materials and Methods: Several lots of IVIG derived from healthy donors in Japan were tested for virus neutralization using single- or multi-cycle virus neutralizing (S-VN or M-VN) assays that evaluate the infection-step associated with HA or the infection and propagation steps associated with HA and NA, respectively. In addition, anti-NA activities were evaluated by inhibiting the enzymatic activity in NAI assays.Results: IVIG lots showed high neutralizing activities against three A/H5N1 strains in M-VN assays, whereas activities in S-VN assays were unstable. In addition, A/H7N2 was also neutralized in S-VN and M-VN assays, with higher activity in M-VN than in S-VN assays. A/H7N1 was neutralized in S-VN and M-VN assays. In contrast, weak or no activity against A/H7N7, A/H7N9, and A/H10N9 was observed in S-VN and M-VN assays. NAI assay results show that IVIG lots had inhibitory activities against N1 and N2; however, N2 activities differed depending on the strain. In contrast, no activities were observed against N7 and N9.Conclusion: These results suggest that IVIG lots have neutralizing activity against avian influenza viruses during the virus propagation step, except for one strain, although no or weak activity was observed during the infection step.Keywords: avian influenza virus, A/H5, A/H7, neutralizing, intravenous immunoglobulin

Published

2021

25. Shedding of rubella virus in postsymptomatic individuals; viral RNA load is a potential indicator to estimate candidate patients excreting infectious rubella virus

Author

Daiki Kanbayashi, Takako Kurata, Atsushi Kaida, Hideyuki Kubo, Seiji P. Yamamoto, Kazutaka Egawa, Yuki Hirai, Kazuma Okada, Yuko Kaida, Ryo Ikemori, Takahiro Yumisashi, Ayami Ito, Takeshi Saito, Yoshihiko Yamaji, Yuka Nishino, Ryosuke Omori, Haruyo Mori, Kazushi Motomura, and Kazuyoshi Ikuta

Subjects

Infectious Diseases, Virology

Published

2023

26. Ongoing rubella epidemic in Osaka, Japan in 2018–2019

Author

Ryo Ikemori, Kazuma Okada, Takako Kurata, Hideki Yoshida, Seiji P. Yamamoto, Kazuyoshi Ikuta, Daiki Kanbayashi, Kazutaka Egawa, Atsushi Kaida, Takahiro Yumisashi, Kazushi Motomura, Hideyuki Kubo, Yuki Hirai, Takanori Hirayama, and Akira Yamamoto

Subjects

Adult, Male, medicine.medical_specialty, Adolescent, Non Theme Issue, Brief-Report, MEDLINE, lcsh:Medicine, Rubella, Young Adult, medicine, Humans, Rubella Vaccine, viruses, Child, Epidemics, Aged, business.industry, lcsh:Public aspects of medicine, rubella, lcsh:R, Infant, Newborn, Infant, lcsh:RA1-1270, General Medicine, Middle Aged, medicine.disease, japan, genotype 1e, Child, Preschool, Family medicine, Female, business, rubella virus

Abstract

A large rubella epidemic is currently ongoing since 2018 in Osaka, Japan. The detected rubella viruses were classified into genotypes 1E lineage 2 and 2B lineage 1. These strains may have been imported from endemic countries, and these viruses spread within the susceptible population.

Published

2021

27. Quantification of a cell-mediated immune response against varicella zoster virus by assessing responder CD4high memory cell proliferation in activated whole blood cultures

Author

Michihiro Takei, Kazuyoshi Ikuta, Masafumi Ohno, Hirotaka Ebina, Ritsuko Koketsu, Toshiomi Okuno, Kazue Hirota, Shinichi Iwamoto, Ahmad M. Haredy, Koichi Yamanishi, and Mitsuyo Kosaka

Subjects

viruses, 030231 tropical medicine, medicine.disease_cause, Flow cytometry, 03 medical and health sciences, 0302 clinical medicine, Antigen, Immunity, medicine, Blood culture, 030212 general & internal medicine, Whole blood, integumentary system, General Veterinary, General Immunology and Microbiology, medicine.diagnostic_test, biology, business.industry, Public Health, Environmental and Occupational Health, Varicella zoster virus, virus diseases, Vaccination, Infectious Diseases, Granzyme, Immunology, biology.protein, Molecular Medicine, business

Abstract

Background Herpes zoster (HZ) is caused by reactivation of a latent varicella zoster virus (VZV). The potential to develop HZ increases with age due to waning of memory cell-mediated immunity (CMI), mainly the CD4 response. Therefore, VZV-CD4-memory T cells (CD4-M) count in blood could serve as a barometer for HZ protection. However, direct quantification of these cells is known to be difficult because they are few in number in the blood. We thus developed a method to measure the proliferation level of CD4-M cells responding to VZV antigen in whole blood culture. Methods Blood samples were collected from 32 children (2–15 years old) with or without a history of varicella infection, 18 young adults (28–45 years old), and 80 elderly (50–86 years old) with a history of varicella infection. The elderly group was vaccinated, and blood samples were taken 2 months and 1 year after VZV vaccination. Then, 1 mL of blood was mixed with VZV, diluted 1/10 in medium, and cultured. CD4-M cells were identified and measured by flow cytometry. Results There was distinct proliferation of CD3+CD4highCD45RA−RO+ (CD4high-M) cells specific to VZV antigen at day 9. The majority of CD4high-M cells had the effector memory phenotype CCR7− and was granzyme B-positive. CD4high-M cells were detected in blood culture from varicella-immune but not varicella-non-immune children. Meanwhile, a higher level of CD4high-M proliferation was observed in young adults than in the elderly. The CD4high-M proliferation level was boosted 2 months after VZV vaccination and maintained for at least 1 year in the elderly. Conclusion Quantifying VZV responder CD4high -M cell proliferation is a convenient way to measure VZV CMI using small blood volumes. Our method can be applied to measure VZV vaccine-induced CMI in the elderly. Clinical study registry numbers: ( www.clinicaltrials.jp ) 173532 and 183985.

Published

2019

28. In vitro antiviral activity of spirotetronate compounds against dengue virus serotype 2

Author

Watanalai Panbangred, Jirayut Euanorasetr, Bungonsiri Intra, Nutthanit Thunmrongsiri, Jitra Limthongkul, Kazuyoshi Ikuta, Takeshi Kurosu, Takuya Nihira, Sukathida Ubol, and Atchareeya A-nuegoonpipat

Subjects

0106 biological sciences, Serotype, 0303 health sciences, Protease, Chemistry, viruses, medicine.medical_treatment, Dengue virus, medicine.disease_cause, 01 natural sciences, Applied Microbiology and Biotechnology, Microbiology, In vitro, 03 medical and health sciences, Viral replication, 010608 biotechnology, medicine, Vero cell, Cytotoxic T cell, Cytotoxicity, 030304 developmental biology

Abstract

Spirotetronate compounds are polyketide secondary metabolites with diverse biological functions, such as antibacterial, antitumor and antiviral activities. Three pure spirotetronate compounds (2EPS-A, -B, -C) isolated from Actinomadura strain 2EPS showed inhibitory activity against dengue virus serotype 2 (DENV-2). 2EPS-A, -B and -C demonstrated the LC50 values of 11.6, 27.5 and 12.0 μg/ml, respectively, in a test of cytotoxicity to Vero cells. The least cytotoxic, 2EPS-B, was further analyzed for its impact on viral propagation in a cell-based replication assay. At a concentration of 6.25 μg/ml, it could reduce the DENV-2 infection in Vero cells by about 94% when cells infected with DENV-2 were exposed to 2EPS-B, whereas direct treatment of DENV-2 with 2EPS-B at the same concentration prior to subsequent infection to Vero cell yielded no inhibition. 2EPS-A, -B an -C showed strong DENV-2 NS2B-NS3 protease inhibition in an in vitro assay, with IC50 values of 1.94 ± 0.18, 1.47 ± 0.15 and 2.51 ± 0.21 μg/ml, respectively. Therefore, the spirotetronate compounds appear to prevent viral replication and viral assembly by inhibition of the viral protease.

Published

2019

29. Two Different Strains of Severe Fever with Thrombocytopenia Syndrome Virus (SFTSV) in North and South Osaka by Phylogenetic Analysis of Evolutionary Lineage: Evidence for Independent SFTSV Transmission

Author

Kazuyoshi Ikuta, Hirono Takabayashi, Tadahiro Sasaki, Ryo Ikemori, Kazutoshi Morisada, Takahiro Yumisashi, Masaru Kinoshita, Kazushi Motomura, and Ikuko Aoyama

Subjects

0301 basic medicine, Phlebovirus, Lineage (genetic), Severe Fever with Thrombocytopenia Syndrome, genotype, 030231 tropical medicine, Reassortment, lcsh:QR1-502, Genome, Viral, lcsh:Microbiology, Evolution, Molecular, 03 medical and health sciences, 0302 clinical medicine, Japan, Virology, Genotype, medicine, Humans, Phylogeny, biology, Phylogenetic tree, SFTS, whole genome, Brief Report, SFTS virus, biology.organism_classification, medicine.disease, Severe fever with thrombocytopenia syndrome, 030104 developmental biology, Infectious Diseases, Infectious disease (medical specialty), RNA, Viral, Severe fever with thrombocytopenia syndrome virus

Abstract

Severe fever with thrombocytopenia syndrome (SFTS) is a novel tick-borne infectious disease, therefore, the information on the whole genome of the SFTS virus (SFTSV) is still limited. This study demonstrates a nearly whole genome of the SFTSV identified in Osaka in 2017 and 2018 by next-generation sequencing (NGS). The evolutionary lineage of two genotypes, C5 and J1, was identified in Osaka. The first case in Osaka belongs to suspect reassortment (L:C5, M:C5, S:C4), the other is genotype J1 (L: J1, M: J1, S: J1) according to the classification by a Japanese group. C5 was identified in China, indicating that C5 identified in this study may be transmitted by birds between China and Japan. This study revealed that different SFTSV genotypes were distributed in two local areas, suggesting the separate or focal transmission patterns in Osaka.

Published

2021

30. Polyethyleneimine-modified resins effectively remove porcine circovirus and cellular prion protein

Author

Natsuki Okaniwa, Teruhide Yamaguchi, Mikihiro Yunoki, Kazuyoshi Ikuta, Kaoru Sakai, Takeru Urayama, Aoyama Shigeyuki, and Eriko Uchida

Subjects

0301 basic medicine, Tris, Circovirus, Chromatography, Molecular mass, Ion exchange, biology, Swine, animal diseases, 030106 microbiology, technology, industry, and agriculture, macromolecular substances, biology.organism_classification, Biological materials, Prion Proteins, 03 medical and health sciences, chemistry.chemical_compound, Porcine circovirus, 030104 developmental biology, chemistry, Virology, Animals, Polyethyleneimine, Prion protein, Pathogen

Abstract

Polyethyleneimine (PEI) possesses various molecular weights (MWs), structures, and virus capture capacities. However, whether PEI can capture porcine circovirus (PCV) and animal cell-derived prion protein (PrPC) that may contaminate source materials is unclear. Therefore, we conducted a feasibility study to assess the effectiveness of PEI in removing PCV and PrPC as a model of pathogenic prions. The removal performance of PCV was evaluated by quantitative PCR using PEIs with various MWs, structures, and ion exchange capacities in Tris (pH 7.5) and acetate (pH 5.5) buffers under neutral (pH 7.5) to acidic (pH 5.5) conditions. Removal performances of PrPC were also evaluated by western blotting using PEIs with various MWs and structures. Tris buffer did not affect the ability of PEI-modified resins to remove PCV, whereas acetate buffer affected removal performances, except those of PEI-10K-Br and PEI-70K-Br, which showed high ion-exchange capacities. PrPC was captured by PEIs with high MWs, especially PEI-70K-Br, which was the most effective. The results of this feasibility study suggested that PEI-modified resin could remove PCV and PrPC. PEI-70K-Br with an ion-exchange capacity of at least 0.3 meq/mL appears suitable as a PEI molecule for pathogen capture or removal of PCV or PrPC from biological materials.

Published

2020

31. Fully Human Monoclonal Antibodies Effectively Neutralizing Botulinum Neurotoxin Serotype B

Author

Kazuyoshi Ikuta, Takuhiro Matsumura, Ryo Misaki, Masahiro Yutani, Kazuhito Fujiyama, Sho Amatsu, Yukako Fujinaga, Tomoko Kohda, and Anariwa Du

Subjects

Serotype, Health, Toxicology and Mutagenesis, lcsh:Medicine, Toxicology, medicine.disease_cause, Neutralization, Epitopes, Mice, Antibody Specificity, SPYMEG, Clostridium botulinum, Neurotoxin, Botulism, Botulinum Toxins, Type A, fully human monoclonal antibody, 0303 health sciences, biology, Chemistry, Antibodies, Monoclonal, Drug Therapy, Combination, Female, Antibody, Protein Binding, therapeutic effect, medicine.drug_class, Monoclonal antibody, Immunoglobulin light chain, Article, preventive effect, 03 medical and health sciences, Neutralization Tests, medicine, Potency, Animals, Humans, 030304 developmental biology, Hybridomas, botulism, 030306 microbiology, Toxin, lcsh:R, neurotoxin, medicine.disease, Virology, Disease Models, Animal, biology.protein, Binding Sites, Antibody, Broadly Neutralizing Antibodies

Abstract

Botulinum neurotoxin (BoNT) is the most potent natural toxin known. Of the seven BoNT serotypes (A to G), types A, B, E, and F cause human botulism. Treatment of human botulism requires the development of effective toxin-neutralizing antibodies without side effects such as serum sickness and anaphylaxis. In this study, we generated fully human monoclonal antibodies (HuMAbs) against serotype B BoNT (BoNT/B1) using a murine&ndash, human chimera fusion partner cell line named SPYMEG. Of these HuMAbs, M2, which specifically binds to the light chain of BoNT/B1, showed neutralization activity in a mouse bioassay (approximately 10 i.p. LD50/100 &micro, g of antibody), and M4, which binds to the C-terminal of heavy chain, showed partial protection. The combination of two HuMAbs, M2 (1.25 &micro, g) and M4 (1.25 &micro, g), was able to completely neutralize BoNT/B1 (80 i.p. LD50) with a potency greater than 80 i.p. LD50/2.5 &micro, g of antibodies, and was effective both prophylactically and therapeutically in the mouse model of botulism. Moreover, this combination showed broad neutralization activity against three type B subtypes, namely BoNT/B1, BoNT/B2, and BoNT/B6. These data demonstrate that the combination of M2 and M4 is promising in terms of a foundation for new human therapeutics for BoNT/B intoxication.

Published

2020

32. Cystargamide B, a cyclic lipodepsipeptide with protease inhibitory activity from Streptomyces sp

Author

Atchareeya A-nuegoonpipat, Takeshi Kurosu, Takuya Nihira, Mitsuki Yoshida, Kazuyoshi Ikuta, Yasuhiro Igarashi, Ousana Boonlucksanawong, Shigeru Kitani, and Watanalai Panbangred

Subjects

0301 basic medicine, Magnetic Resonance Spectroscopy, Stereochemistry, medicine.medical_treatment, Molecular Conformation, Spectrometry, Mass, Fast Atom Bombardment, Streptomyces, 03 medical and health sciences, Residue (chemistry), Zingiberaceae, Depsipeptides, Drug Discovery, medicine, Kaempferia galanga, Protease Inhibitors, Pharmacology, chemistry.chemical_classification, Protease, biology, Fatty acid, Nuclear magnetic resonance spectroscopy, Dengue Virus, Fast atom bombardment, biology.organism_classification, Amino acid, 030104 developmental biology, chemistry, Rhizome

Abstract

We identified a new cyclic lipodepsipeptide, cystargamide B (1), from the mycelial extract of a Kaempferia galanga rhizome-derived actinomycete strain, Streptomyces sp. PB013. The planar structure was elucidated based on high resolution fast-atom bombardment mass spectrometry (HRFABMS) spectroscopy and one-dimensional (1D) and two-dimensional (2D) nuclear magnetic resonance (NMR) spectroscopic data. The absolute configurations of the constituent amino acids were determined using advanced Marfey's method. Cystargamide B (1) includes rare structural units: a 5-hydroxytryptophan residue and a 2,3-epoxy fatty acid side chain. Notably, cystargamide B (1) inhibited the protease activity of the NS2B/NS3 complex from dengue virus.

Published

2018

33. Human protective monoclonal antibodies against the HA stem of group 2 HAs derived from an H3N2 virus-infected human

Author

Tadahiro Sasaki, Yoshihiro Kawaoka, Kazuyoshi Ikuta, Seiya Yamayoshi, Mutsumi Ito, and Ryuta Uraki

Subjects

0301 basic medicine, Microbiology (medical), medicine.drug_class, 030106 microbiology, Hemagglutinin Glycoproteins, Influenza Virus, Antibodies, Viral, Monoclonal antibody, medicine.disease_cause, Article, Germline, Virus, Epitope, Epitopes, 03 medical and health sciences, Neutralization Tests, In vivo, medicine, Influenza A virus, Animals, Humans, Mice, Inbred BALB C, biology, Influenza A Virus, H3N2 Subtype, Antibodies, Monoclonal, Antibodies, Neutralizing, Virology, In vitro, HEK293 Cells, 030104 developmental biology, Infectious Diseases, Immunoglobulin G, Mutation, biology.protein, Female, Antibody

Abstract

Objectives Broadly reactive human monoclonal antibodies against the HA stem of influenza A virus are being developed as therapeutic agents as well as to understand the epitopes that are essential for a universal influenza virus vaccine. Methods We isolated and characterized two hetero-reactive human monoclonal antibodies from an H3N2 virus-infected human. Results These antibodies, which are predominantly bound to the HA stem of group 2 HAs, used IGHV3-66 and IGHV4-38-2 germline genes, respectively. They possessed in vitro neutralizing ability, and in vivo protective efficacy against lethal infection with H3N2 or H7N9 virus. Escape mutations revealed that one of the protective antibodies recognized the α-helix A of HA2, and the other recognized the C-terminal portion of the fusion peptide and the β-sheet that precedes the α-helix A of HA2. Conclusions Of many human protective monoclonal antibodies against the HA stem, two human protective monoclonal antibodies were isolated in this study that predominantly recognize epitopes on the HA stem of group 2 and use unique IGHV3-66 and IGHV4-38-2 germline genes.

Published

2018

34. Protective effects ofin vivo-expressed autotransporters againstBordetella pertussisinfection

Author

Koichiro Suzuki, Aya Fukui-Miyazaki, Hiroyuki Abe, Kazuyoshi Ikuta, Naoaki Shinzawa, Yasuhiko Horiguchi, Keisuke Ishigaki, and Keiji Nakamura

Subjects

0301 basic medicine, Bordetella pertussis, biology, Immunology, Respiratory disease, biology.organism_classification, medicine.disease, Microbiology, respiratory tract diseases, 03 medical and health sciences, 030104 developmental biology, medicine.anatomical_structure, Immunization, Antigen, Virology, medicine, Nasal administration, Whooping cough, Autotransporters, Respiratory tract

Abstract

Bordetella pertussis causes whooping cough, a severe and prolonged respiratory disease that results in high morbidity and mortality rates, particularly in developing countries. The number of whooping cough cases is increasing in many countries despite high vaccine coverage. Causes for the re-emergence of the disease include the limited duration of protection conferred by the acellular pertussis vaccines (aP) and pathogenic adaptations that involve antigenic divergence from vaccine strains. Therefore, current vaccines need to be improved. In the present study, we focused on five autotransporters: SphB1, BatB, SphB2, Phg, and Vag8, which were previously found to be expressed by B. bronchiseptica during the course of infection in rats, and examined their protective efficiencies as vaccine antigens. The passenger domains of these proteins were produced in recombinant forms and used as antigens. An intranasal murine challenge assay showed that immunization with a mixture of SphB1 and Vag8 (SV) significantly reduced bacterial load in the lower respiratory tract and combination of aP and SV yield synergistic effects of protection against B. pertussis infection, implying that these antigens have potential as components to improve the currently available acellular pertussis vaccine.

Published

2017

35. A Broadly Reactive Human Anti-hemagglutinin Stem Monoclonal Antibody That Inhibits Influenza A Virus Particle Release

Author

Atsuhiro Yasuhara, Kohei Oishi, Mutsumi Ito, Kazuyoshi Ikuta, Sumiho Nakatsu, Ryuta Uraki, Maki Kiso, Seiya Yamayoshi, Tadahiro Sasaki, and Yoshihiro Kawaoka

Subjects

0301 basic medicine, medicine.drug_class, 030106 microbiology, Antibody Affinity, lcsh:Medicine, Hemagglutinin (influenza), CHO Cells, Virus Replication, Monoclonal antibody, medicine.disease_cause, General Biochemistry, Genetics and Molecular Biology, Epitope, Virus, Madin Darby Canine Kidney Cells, Epitopes, Mice, HA stem, 03 medical and health sciences, Cricetulus, Dogs, Antigen, Viral entry, Cricetinae, medicine, Influenza A virus, Animals, Humans, Cells, Cultured, Virus Release, lcsh:R5-920, biology, lcsh:R, Antibodies, Monoclonal, General Medicine, Human monoclonal antibody, Virology, HEK293 Cells, Hemagglutinins, 030104 developmental biology, Viral replication, Broadly reactive, biology.protein, lcsh:Medicine (General), HeLa Cells, Research Paper

Abstract

Many broadly reactive human monoclonal antibodies against the hemagglutinin (HA) stem of influenza A virus have been developed for therapeutic applications. These antibodies typically inhibit viral entry steps, especially the HA conformational change that is required for membrane fusion. To better understand the mechanisms by which such antibodies inhibit viral replication, we established broadly reactive human anti-HA stem antibodies and determined the properties of these antibodies by examining their reactivity with 18 subtypes of HA, evaluating their in vivo protective efficacy, identifying their epitopes, and characterizing their inhibitory mechanisms. Among the eight human monoclonal antibodies we generated, which recognized at least 3 subtypes of the soluble HA antigens tested, clone S9-1-10/5-1 reacted with 18 subtypes of HA and protected mice from lethal infection with H1N1pdm09, H3N2, H5N1, and H7N9 viruses. This antibody recognized the HA2 helix A in the HA stem, and inhibited virus particle release from infected cells but did not block viral entry completely. These results show that broadly reactive human anti-HA stem antibodies can exhibit protective efficacy by inhibiting virus particle release. These findings expand our knowledge of the mechanisms by which broadly reactive stem-targeting antibodies inhibit viral replication and provide valuable information for universal vaccine development., Highlights • A broadly mouse-protective anti-HA stem antibody, S9-1-10/5-1, was isolated. • S9-1-10/5-1 mainly inhibited virus release rather than virus entry. • S9-1-10/5-1 tethers virions via crosslinking HA molecules between neighboring virions. Broadly reactive human monoclonal antibodies against the influenza HA stem have received attention because of their potential utility against multiple HA subtypes. Some of these antibodies inhibit virus entry and/or protect mice via antibody-dependent cellular cytotoxicity. Here, we identified a human monoclonal antibody that suppresses virus propagation in vitro and in vivo by primarily inhibiting virus particle release. This finding provides another inhibitory mechanism of action for the anti-HA stem antibodies, indicating that the anti-HA stem antibodies could be potent anti-virals due to their pluripotency.

Published

2017

36. Neutralizing activities against seasonal influenza viruses in human intravenous immunoglobulin

Author

Kazue Hirota, Hiroyuki Onodera, Kazuyoshi Ikuta, Yoshinobu Okuno, Takeru Urayama, Kazuhiro Maeda, Kazuo Takahashi, Mikihiro Yunoki, Katsuro Hagiwara, and Ritsuko Kubota-Koketsu

Subjects

0301 basic medicine, Antigenicity, viruses, Population, Virus, Neutralization, 03 medical and health sciences, 0302 clinical medicine, Rheumatology, Antigen, vaccine, Immunology and Allergy, Medicine, Pharmacology (medical), Targets and Therapy [Biologics], 030212 general & internal medicine, education, Original Research, IVIG, education.field_of_study, Hemagglutination assay, biology, business.industry, Gastroenterology, virus diseases, seasonal, neutralization, Virology, Titer, 030104 developmental biology, Oncology, biology.protein, Antibody, business, influenza

Abstract

Hiroyuki Onodera,1 Takeru Urayama,2 Kazue Hirota,3 Kazuhiro Maeda,3 Ritsuko Kubota-Koketsu,3,4 Kazuo Takahashi,5 Katsuro Hagiwara,6 Yoshinobu Okuno,3 Kazuyoshi Ikuta,3,4 Mikihiro Yunoki,2,4,6 1Medical Information Department, 2Research and Development Division, Japan Blood Products Organization, Tokyo, 3Research and Development Division, The Research Foundation for Microbial Diseases of Osaka University, Kagawa, 4Former Department of Virology, Research Institute for Microbial Diseases, Osaka University, 5Virology Division, Department of Infectious Diseases, Osaka Prefectural Institute of Public Health, Osaka, 6Pathogenic Risk Evaluation, Graduate School of Veterinary Medicine, Rakuno Gakuen University, Hokkaido, Japan Abstract: Influenza viruses A/H1N1, A/H3N2, and B are known seasonal viruses that undergo annual mutation. Intravenous immunoglobulin (IVIG) contains anti-seasonal influenza virus globulins. Although the virus-neutralizing (VN) titer is an indicator of protective antibodies, changes in this titer over extended time periods have yet to be examined. In this study, variations in hemagglutination inhibition (HI) and VN titers against seasonal influenza viruses in IVIG lots over extended time periods were examined. In addition, the importance of monitoring the reactivity of IVIG against seasonal influenza viruses with varying antigenicity was evaluated. A/H1N1, A/H3N2, and B influenza virus strains and IVIG lots manufactured from 1999 to 2014 were examined. The HI titer was measured by standard methods. The VN titer was measured using a micro-focus method. IVIG exhibited significant HI and VN titers against all investigated strains. Our results suggest that the donor population maintains both specific and cross-reactive antibodies against seasonal influenza viruses, except in cases of pandemic viruses, despite major antigen changes. The titers against seasonal influenza vaccine strains, including past strains, were stable over short time periods but increased slowly over time. Keywords: IVIG, influenza, seasonal, neutralization, vaccine

Published

2017

37. Quantification of a cell-mediated immune response against varicella zoster virus by assessing responder CD4

Author

Ahmad M, Haredy, Michihiro, Takei, Shin-Ichi, Iwamoto, Masafumi, Ohno, Mitsuyo, Kosaka, Kazue, Hirota, Ritsuko, Koketsu, Toshiomi, Okuno, Kazuyoshi, Ikuta, Koichi, Yamanishi, and Hirotaka, Ebina

Subjects

Adult, Aged, 80 and over, CD4-Positive T-Lymphocytes, Male, Immunity, Cellular, Vaccination, Middle Aged, Flow Cytometry, Vaccines, Attenuated, Herpes Zoster, Blood Culture, Herpes Zoster Vaccine, Humans, Female, Aged, Cell Proliferation

Abstract

Herpes zoster (HZ) is caused by reactivation of a latent varicella zoster virus (VZV). The potential to develop HZ increases with age due to waning of memory cell-mediated immunity (CMI), mainly the CD4 response. Therefore, VZV-CD4-memory T cells (CD4-M) count in blood could serve as a barometer for HZ protection. However, direct quantification of these cells is known to be difficult because they are few in number in the blood. We thus developed a method to measure the proliferation level of CD4-M cells responding to VZV antigen in whole blood culture.Blood samples were collected from 32 children (2-15 years old) with or without a history of varicella infection, 18 young adults (28-45 years old), and 80 elderly (50-86 years old) with a history of varicella infection. The elderly group was vaccinated, and blood samples were taken 2 months and 1 year after VZV vaccination. Then, 1 mL of blood was mixed with VZV, diluted 1/10 in medium, and cultured. CD4-M cells were identified and measured by flow cytometry.There was distinct proliferation of CD3Quantifying VZV responder CD4

Published

2019

38. In vitro antiviral activity of spirotetronate compounds against dengue virus serotype 2

Author

Jirayut, Euanorasetr, Bungonsiri, Intra, Nutthanit, Thunmrongsiri, Jitra, Limthongkul, Sukathida, Ubol, Atchareeya, Anuegoonpipat, Takeshi, Kurosu, Kazuyoshi, Ikuta, Takuya, Nihira, and Watanalai, Panbangred

Subjects

Actinobacteria, Inhibitory Concentration 50, Polyketides, Chlorocebus aethiops, Animals, Protease Inhibitors, Dengue Virus, Serogroup, Virus Replication, Antiviral Agents, Vero Cells

Abstract

Spirotetronate compounds are polyketide secondary metabolites with diverse biological functions, such as antibacterial, antitumor and antiviral activities. Three pure spirotetronate compounds (2EPS-A, -B, -C) isolated from Actinomadura strain 2EPS showed inhibitory activity against dengue virus serotype 2 (DENV-2). 2EPS-A, -B and -C demonstrated the LC

Published

2019

39. Recombinant production and characterization of human anti-influenza virus monoclonal antibodies identified from hybridomas fused with human lymphocytes

Author

Hiroyuki Kajiura, Ryo Misaki, Natsuko Fukura, Kazuyoshi Ikuta, Ken-ichiro Ono, Kazuhito Fujiyama, Takao Ohashi, Masatoshi Momota, Mayo Yasugi, Ritsuko Kubota-Koketsu, and Tadahiro Sasaki

Subjects

0301 basic medicine, Glycan, medicine.drug_class, Bioengineering, Antibodies, Viral, Monoclonal antibody, Applied Microbiology and Biotechnology, Human Immunoglobulin G, Virus, law.invention, Cell Fusion, 03 medical and health sciences, 0302 clinical medicine, law, Cricetinae, medicine, Animals, Humans, Secretion, Lymphocytes, Pharmacology, Hybridomas, General Immunology and Microbiology, biology, Chinese hamster ovary cell, Antibodies, Monoclonal, General Medicine, Antibodies, Neutralizing, Virology, Molecular biology, carbohydrates (lipids), Influenza B virus, 030104 developmental biology, Influenza A virus, Immunoglobulin G, 030220 oncology & carcinogenesis, biology.protein, Recombinant DNA, Antibody, Biotechnology

Abstract

In previous studies, hybridomas producing human immunoglobulin G, the antibodies 5E4 and 5A7 against influenza A and B virus were established using a novel human lymphocyte fusion partner, SPYMEG. In the present study, we succeeded in achieving the recombinant production and secretion of 5E4 and 5A7 in Chinese hamster ovary cells. Our N-glycan analysis by intact-mass detection and liquid chromatography mass spectrometry showed that recombinant 5E4 and 5A7 have one N-glycan and the typical mammalian-type N-glycan structures similar to those in hybridomas. However, the glycan distribution was slightly different among these antibodies. The amount of high-mannose-type structures was under 10% of the total N-glycans of recombinant 5E4 and 5A7, compared to 20% of the 5E4 and 5A7 produced in hybridomas. The amount of galactosylated N-glycans was increased in recombinants. Approximately 80% of the N-glycans of all antibodies was fucosylated, and no sialylated N-glycan was found. Recombinant 5E4 and 5A7 neutralized pandemic influenza A virus specifically, and influenza B virus broadly, quite similar to the 5E4 and 5A7 produced in hybridomas, respectively. Here we demonstrated that recombinants of antibodies identified from hybridomas fused with SPYMEG have normal N-glycans and that their neutralizing activities bear comparison with those of the original antibodies.

Published

2016

40. Neutralizing activities of human immunoglobulin derived from donors in Japan against mosquito-borne flaviviruses, Japanese encephalitis virus, West Nile virus, and dengue virus

Author

Takeshi Kurosu, Yoshinobu Okuno, Ritsuko Koketsu, Kazuyoshi Ikuta, Kazuo Takahashi, and Mikihiro Yunoki

Subjects

0301 basic medicine, viruses, Population, Short Report, Dengue virus, medicine.disease_cause, Neutralization, Virus, Dengue fever, 03 medical and health sciences, 0302 clinical medicine, Rheumatology, medicine, Immunology and Allergy, Targets and Therapy [Biologics], Pharmacology (medical), intravenous immuno-globulin, education, 030203 arthritis & rheumatology, education.field_of_study, dengue virus, biology, business.industry, Gastroenterology, virus diseases, neutralization, Japanese encephalitis, medicine.disease, Virology, nervous system diseases, Japanese encephalitis virus, 030104 developmental biology, Oncology, biology.protein, Antibody, business, West Nile virus, Encephalitis

Abstract

Mikihiro Yunoki,1-3 Takeshi Kurosu,2 Ritsuko Kubota Koketsu,2,4 Kazuo Takahashi,5 Yoshinobu Okuno,4 Kazuyoshi Ikuta2,4 1Research and Development Division, Japan Blood Products Organization, Tokyo, 2Department of Virology, Research Institute for Microbial Diseases, Osaka University, Osaka, 3Pathogenic Risk Evaluation, Graduate School of Veterinary Medicine, Rakuno Gakuen University, Hokkaido, 4Research and Development Division, The Research Foundation for Microbial Diseases of Osaka University, Kagawa, 5Osaka Prefectural Institute of Public Health, Osaka, Japan Abstract: Japanese encephalitis virus (JEV), West Nile virus (WNV), and dengue virus (DenV) are causal agents of Japanese encephalitis, West Nile fever, and dengue fever, respectively. JEV is considered to be indigenized and widespread in Japan, whereas WNV and DenV are not indigenized in Japan. Globulin products seem to reflect the status of the donor population according to antivirus neutralization activity. However, the anti-JEV, -WNV, and -DenV neutralization activities of globulin products derived from donors in Japan have not been clarified. Furthermore, potential candidates for the development of an effective immunotherapeutic drug for encephalitis caused by JEV, WNV, or DenV have also not been identified. Therefore, the aim of this study was to determine the overall status of the donor population in Japan based on globulin products by evaluating anti-JEV, -WNV, and -DenV neutralizing activities of intravenous immunoglobulin. Overall, intravenous immunoglobulin products showed stable neutralizing activity against JEV but showed no or only weak activity against WNV or DenV. These results suggest that the epidemiological level against WNV and DenV in the donor population of Japan is still low, suggesting that these viruses are not yet indigenized. In addition, JEV vaccinations and/or infections in the donor population do not induce a cross-reactive antibody against WNV. Keywords: Japanese encephalitis virus, West Nile virus, dengue virus, intravenous immunoglobulin, neutralization

Published

2016

41. Capture of dengue viruses using antibody-integrated graphite-encapsulated magnetic beads produced using gas plasma technology

Author

Akikazu Sakudo, Masaaki Nagatsu, Kazuyoshi Ikuta, Tadahiro Sasaki, Han Chou, and Anchu Viswan

Subjects

0301 basic medicine, Cancer Research, virus capture, Plasma Gases, viruses, 02 engineering and technology, Dengue virus, Biology, medicine.disease_cause, Immunomagnetic separation, Antibodies, Viral, Biochemistry, Virus, Dengue fever, Cell Line, 03 medical and health sciences, gas plasma, antibody, Genetics, Gas plasma, medicine, Animals, Humans, Molecular Biology, Ammonia gas, graphite, Immunomagnetic Separation, virus diseases, Articles, biochemical phenomena, metabolism, and nutrition, Dengue Virus, 021001 nanoscience & nanotechnology, medicine.disease, Virology, dengue, 030104 developmental biology, Oncology, biology.protein, Molecular Medicine, Nanoparticles, Antibody, 0210 nano-technology, Genomic rna, virus concentration

Abstract

Despite significant advances in medicine, global health is threatened by emerging infectious diseases caused by a number of viruses. Dengue virus (DENV) is a mosquito‑borne virus, which can be transmitted to humans via mosquito vectors. Previously, the Ministry of Health, Labour and Welfare in Japan reported the country's first domestically acquired case of dengue fever for almost 70 years. To address this issue, it is important to develop novel technologies for the sensitive detection of DENV. The present study reported on the development of plasma-functionalized, graphite-encapsulated magnetic nanoparticles (GrMNPs) conjugated with anti-DENV antibody for DENV capture. Radiofrequency wave‑excited inductively‑coupled Ar and ammonia gas plasmas were used to introduce amino groups onto the surface of the GrMNPs. The GrMNPs were then conjugated with an antibody against DENV, and the antibody‑integrated magnetic beads were assessed for their ability to capture DENV. Beads incubated in a cell culture medium of DENV‑infected mosquito cells were separated from the supernatant by applying a magnetic field and were then washed. The adsorption of DENV serotypes 1‑4 onto the beads was confirmed using reverse transcription‑polymerase chain reaction, which detected the presence of DENV genomic RNA on the GrMNPs. The methodology described in the present study, which employed the plasma-functionalization of GrMNPs to enable antibody‑integration, represents a significant improvement in the detection of DENV.

Published

2016

42. Evaluation of the fusion partner cell line SPYMEG for obtaining human monoclonal antibodies against influenza B virus

Author

Tadahiro Sasaki, Mutsumi Ito, Ryuta Uraki, Priyanka Soni, Kazuyoshi Ikuta, Yoshihiro Kawaoka, Kiyoko Iwatsuki-Horimoto, Toru Takenaga, Seiya Yamayoshi, and Atsuhiro Yasuhara

Subjects

0301 basic medicine, medicine.drug_class, Hemagglutinin (influenza), Hemagglutinin Glycoproteins, Influenza Virus, Biology, Monoclonal antibody, Antibodies, Viral, Peripheral blood mononuclear cell, Epitope, Virus, hybridoma, Cell Line, 03 medical and health sciences, Mice, Immune system, Virology, SPYMEG, medicine, Animals, Humans, Hybridomas, General Veterinary, Full Paper, Antibodies, Monoclonal, influenza B virus, 030104 developmental biology, Cell culture, biology.protein, Leukocytes, Mononuclear, Hybridoma technology, human monoclonal antibody

Abstract

Influenza B virus has been known to infect humans and other animals, including seals. Vaccination efficacy varies across seasons. Human monoclonal antibodies (mAbs) can be useful for developing novel vaccines, guided by epitope analysis, and can be used therapeutically. Hybridoma technology has been used to make mAbs. Here we evaluated SPYMEG as a fusion partner cell line for human mAb generation specific to influenza B hemagglutinin (HA). SPYMEG is a human/murine myeloma partner cell line that has previously been used to generate human mAbs that recognize the HA of influenza A and B viruses. Peripheral blood mononuclear cells were obtained from 16 volunteers, previously vaccinated with the 2014-2015 trivalent seasonal influenza vaccine, and were fused with SPYMEG to yield hybridomas. The resulting hybridomas were screened for antigen-specific antibody secretion and cloned by limiting dilution. We obtained 32 stable clones secreting anti-influenza B HA human IgG, although most of these clones were obtained from one volunteer (SeaV-29) who had a robust immune response. We conclude that SPYMEG is a good fusion partner cell line, although cloning by limiting dilution may lead to significant loss of hybridomas.

Published

2018

43. Diversity of antigenic mutants of influenza A(H1N1)pdm09 virus escaped from human monoclonal antibodies

Author

Kazuyoshi Ikuta, Ryuta Uraki, Shinya Yamada, Yoshihiro Kawaoka, Mutsumi Ito, Tadahiro Sasaki, Emi Takashita, Yuko Sakai-Tagawa, Priyanka Soni, Atsuhiro Yasuhara, Kiyoko Iwatsuki-Horimoto, Seiya Yamayoshi, Toru Takenaga, and Chiharu Kawakami

Subjects

0301 basic medicine, medicine.drug_class, viruses, Glutamine, 030106 microbiology, Mutant, lcsh:Medicine, Hemagglutinin Glycoproteins, Influenza Virus, Monoclonal antibody, medicine.disease_cause, Antigenic drift, Virus, Article, 03 medical and health sciences, Influenza A Virus, H1N1 Subtype, Antigen, Influenza, Human, medicine, Influenza A virus, Humans, Amino Acid Sequence, lcsh:Science, Epidemics, Antigens, Viral, Mutation, Multidisciplinary, biology, Lysine, lcsh:R, Antibodies, Monoclonal, Genetic Variation, Virology, Antigenic Variation, 030104 developmental biology, Amino Acid Substitution, biology.protein, lcsh:Q, Antibody

Abstract

Since the 2017 Southern Hemisphere influenza season, the A(H1N1)pdm09-like virus recommended for use in the vaccine was changed because human, but not ferret, sera distinguish A(H1N1)pdm09 viruses isolated after 2013 from the previously circulating strains. An amino acid substitution, lysine to glutamine, at position 166 (H3 numbering) in the major antigenic site of HA was reported to be responsible for the antigenic drift. Here, we obtained two anti-A(H1N1)pdm09 HA monoclonal antibodies that failed to neutralize viruses isolated after 2013 from a vaccinated volunteer. Escape mutations were identified at position 129, 165, or 166 in the major antigenic site of HA. Competitive growth of the escape mutant viruses with the wild-type virus revealed that some escape mutants possessing an amino acid substitution other than K166Q showed superior growth to that of the wild-type virus. These results suggest that in addition to the K166Q mutation that occurred in epidemic strains, other HA mutations can confer resistance to antibodies that recognize the K166 area, leading to emergence of epidemic strains with such mutations.

Published

2017

44. General applicability and reliability of immuno-chromatography-based RDT kits for POCT at clinics

Author

Ritsuko Kubota-Koketsu, Kazuyoshi Ikuta, and Tadahiro Sasaki

Subjects

business.industry, Point-of-care testing, Medicine, business, Reliability (statistics), Reliability engineering

Published

2015

45. Human monoclonal antibodies with broad-spectrum neutralizing activity against influenza viruses

Author

Kazuyoshi Ikuta, Yang Pan, Ririn Ramadhany, and Tadahiro Sasaki

Subjects

Broad spectrum, medicine.drug_class, medicine, Biology, Monoclonal antibody, Virology

Published

2015

46. Avian Influenza Virus Infection of Immortalized Human Respiratory Epithelial Cells Depends upon a Delicate Balance between Hemagglutinin Acid Stability and Endosomal pH

Author

Hisataka Maruyama, Taisuke Masuda, Kazuyoshi Ikuta, Madiha S. Ibrahim, Takaaki Nakaya, Yohei Watanabe, Tomo Daidoji, Tomoyuki Ohba, Ayae Honda, Fumihito Arai, and Mayo Yasugi

Subjects

Endosome, animal diseases, Cell, Virulence, Hemagglutinin (influenza), Hemagglutinin Glycoproteins, Influenza Virus, Receptors, Cell Surface, Endosomes, Respiratory Mucosa, Biology, medicine.disease_cause, Microbiology, Biochemistry, Virus, Cell Line, Birds, Dogs, Influenza, Human, medicine, Animals, Humans, Molecular Biology, Tropism, Infectivity, Influenza A Virus, H5N1 Subtype, Protein Stability, virus diseases, Cell Biology, Hydrogen-Ion Concentration, Virus Internalization, Virology, Influenza A virus subtype H5N1, Clone Cells, medicine.anatomical_structure, Influenza in Birds, biology.protein

Abstract

The highly pathogenic avian influenza (AI) virus, H5N1, is a serious threat to public health worldwide. Both the currently circulating H5N1 and previously circulating AI viruses recognize avian-type receptors; however, only the H5N1 is highly infectious and virulent in humans. The mechanism(s) underlying this difference in infectivity remains unclear. The aim of this study was to clarify the mechanisms responsible for the difference in infectivity between the current and previously circulating strains. Primary human small airway epithelial cells (SAECs) were transformed with the SV40 large T-antigen to establish a series of clones (SAEC-Ts). These clones were then used to test the infectivity of AI strains. Human SAEC-Ts could be broadly categorized into two different types based on their susceptibility (high or low) to the viruses. SAEC-T clones were poorly susceptible to previously circulating AI but were completely susceptible to the currently circulating H5N1. The hemagglutinin (HA) of the current H5N1 virus showed greater membrane fusion activity at higher pH levels than that of previous AI viruses, resulting in broader cell tropism. Moreover, the endosomal pH was lower in high susceptibility SAEC-T clones than that in low susceptibility SAEC-T clones. Taken together, the results of this study suggest that the infectivity of AI viruses, including H5N1, depends upon a delicate balance between the acid sensitivity of the viral HA and the pH within the endosomes of the target cell. Thus, one of the mechanisms underlying H5N1 pathogenesis in humans relies on its ability to fuse efficiently with the endosomes in human airway epithelial cells.

Published

2015

47. VII. Next Generation Pneumococcal Vaccine

Author

Kazuyoshi Ikuta and Yukihiro Akeda

Subjects

Pneumococcal Vaccines, Pediatrics, medicine.medical_specialty, Pneumococcal vaccine, business.industry, MEDLINE, medicine, Humans, General Medicine, business

Published

2015

48. Construction of a high-yield dengue virus by replacing nonstructural proteins 3-4B without increasing virulence

Author

Magot Diata Omokoko, Kazuyoshi Ikuta, Sabar Pambudi, Supranee Phanthanawiboon, Wataru Kamitani, Keiko Hanabara, Takeshi Kurosu, and Atchareeya A-nuegoonpipat

Subjects

0301 basic medicine, viruses, Biophysics, Virulence, Dengue virus, Biology, Viral Nonstructural Proteins, medicine.disease_cause, Biochemistry, Virus, Dengue fever, 03 medical and health sciences, medicine, Molecular Biology, Recombination, Genetic, NS3, Attenuated vaccine, virus diseases, Cell Biology, biochemical phenomena, metabolism, and nutrition, Dengue Virus, Viral Load, medicine.disease, Virology, Vaccination, 030104 developmental biology, Genetic Enhancement, Viral replication, Batch Cell Culture Techniques

Abstract

Producing virus at high yield is critically important for development of whole virion inactivated vaccines or live attenuated vaccines. Most dengue virus (DENV) clinical isolates, however, replicate at low levels in cultured cells, which limits their use for vaccine development. The present study examined differences between low-replicating DENV clinical isolates and high-replicating laboratory strains with the aim of engineering high-yield DENV clinical isolates. Construction of a series of recombinant chimeric viruses derived from a high-replicating laboratory DENV type 4 (DENV-4) H241 strain and a clinical isolate revealed that the NS3-NS4B region of H241 conferred a replication advantage in cultured cells. Furthermore, northern blot analysis revealed that this advantage was due to more efficient synthesis of viral RNA. Importantly, replacement of the NS3-NS4B region of H241 did not increase virulence in mice, suggesting that viral production can be increased safely. This study provided information that will facilitate engineering of safe and high-yield viruses that can be used for vaccine development.

Published

2017

49. Protective effects of in vivo-expressed autotransporters against Bordetella pertussis infection

Author

Koichiro, Suzuki, Naoaki, Shinzawa, Keisuke, Ishigaki, Keiji, Nakamura, Hiroyuki, Abe, Aya, Fukui-Miyazaki, Kazuyoshi, Ikuta, and Yasuhiko, Horiguchi

Subjects

Pertussis Vaccine, Antigens, Bacterial, Mice, Inbred BALB C, Type V Secretion Systems, Whooping Cough, Respiratory System, Serine Endopeptidases, Vaccination, Antibodies, Bacterial, Antigenic Variation, Bacterial Load, Bordetella pertussis, Mice, Bacterial Proteins, Animals, Female

Abstract

Bordetella pertussis causes whooping cough, a severe and prolonged respiratory disease that results inhas high morbidity and mortality rates, particularly in developing countries. The number incidence of whooping cough cases is increasing in many countries despite high vaccine coverage. Causes for the re-emergence of the disease include the limited duration of protection conferred by the acellular pertussis vaccines (aP)s and pathogenic adaptations that involve antigenic divergence from vaccine strains. Therefore, current vaccines therefore need to be improved. In the present study, we focused on five autotransporters: namely SphB1, BatB, SphB2, Phg, and Vag8, which were previously found to be expressed by B. bronchiseptica during the course of infection in rats and examined their protective efficiencies as vaccine antigens. The passenger domains of these proteins were produced in recombinant forms and used as antigens. An intranasal murine challenge assay showed that immunization with a mixture of SphB1 and Vag8 (SV) significantly reduced bacterial load in the lower respiratory tract and a combination of aP and SV acts synergistically in effects of conferring protection against B. pertussis infection, implying that these antigens have potential as components to for improvinge th the currently available acellular pertussis vaccine.

Published

2017

50. A novel immunochromatographic system for easy-to-use detection of group 1 avian influenza viruses with acquired human-type receptor binding specificity

Author

Kazuyoshi Ikuta, Kouichi Morita, Takaaki Nakaya, Toshihiro Ito, Hiroaki Hiramatsu, Tsukasa Hayashi, Kosuke Soda, Takashi Suzuki, Hoang Vu Mai Phuong, Yasuo Suzuki, Yoshinobu Okuno, Tetsuo Ito, Masaoki Yamaoka, Yasuha Arai, Nongluk Sriwilaijaroen, Laksmi Wulandari, Yohei Watanabe, Tomo Daidoji, Nguyen Le Khanh Hang, Le Quynh Mai, Madiha S. Ibrahim, Emmanuel Djoko Poetranto, Tadanobu Takahashi, Ritsuko Kubota-Koketsu, Tetsu Yamashiro, Hak Hotta, and Kozue Hotta

Subjects

H5N1 avian influenza virus, Group 1 influenza A virus, Hemagglutination, viruses, Biomedical Engineering, Biophysics, Detection of receptor binding specificity, Hemagglutinin Glycoproteins, Influenza Virus, Pandemic potential, medicine.disease_cause, Virus, Article, Chromatography, Affinity, Birds, chemistry.chemical_compound, Influenza, Human, Electrochemistry, medicine, Animals, Humans, Sialylglycopolymer, Reagent Strips, biology, Immunochromatographic strip test, Influenza A Virus, H5N1 Subtype, General Medicine, Equipment Design, Virology, Influenza A virus subtype H5N1, Sialic acid, Titer, chemistry, Influenza A virus, Biotinylation, Influenza in Birds, biology.protein, Antibody, Biotechnology, Avidin

Abstract

A switch of viral hemagglutinin receptor binding specificity from bird-type α2,3- to human-type α2,6-linked sialic acid is necessary for an avian influenza virus to become a pandemic virus. In this study, an easy-to-use strip test to detect receptor binding specificity of influenza virus was developed. A biotinylated anti-hemagglutinin antibody that bound a broad range of group 1 influenza A viruses and latex-conjugated α2,3 (blue) and α2,6 (red) sialylglycopolymers were used in an immunochromatographic strip test, with avidin and lectin immobilized on a nitrocellulose membrane at test and control lines, respectively. Accumulation of a sialylglycopolymer–virus–antibody complex at the test line was visualized by eye. The strip test could be completed in 30 min and did not require special equipment or skills, thereby avoiding some disadvantages of current methods for analyzing receptor binding specificity of influenza virus. The strip test could detect the receptor binding specificity of a wide range of influenza viruses, as well as small increases in the binding affinity of variant H5N1 viruses to α2,6 sialylglycans at viral titers >128 hemagglutination units. The strip test results were in agreement with those of ELISA virus binding assays, with correlations >0.95. In conclusion, the immunochromatographic strip test developed in this study should be useful for monitoring potential changes in the receptor binding specificity of group 1 influenza A viruses in the field., Highlights • A novel immunochromatographic strip test system was developed. • The strip test was developed to detect influenza virus receptor binding specificity. • The strip test was applicable to a broad range of group 1 influenza A viruses. • The strip detected faint increases in human-type specificity of variant H5N1 viruses. • The system could be applied for easy monitoring the viral pandemic potential.

Published

2014