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Dive into the research topics where Seiya Harada is active.

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Featured researches published by Seiya Harada.


Journal of Medical Virology | 2009

Surveillance of pathogens in outpatients with gastroenteritis and characterization of sapovirus strains between 2002 and 2007 in Kumamoto Prefecture, Japan.

Seiya Harada; Mineyuki Okada; Shunsuke Yahiro; Koichi Nishimura; Shigeru Matsuo; Jiro Miyasaka; Ryuichi Nakashima; Yasushi Shimada; Takehiko Ueno; Shigeru Ikezawa; Kuniko Shinozaki; Kazuhiko Katayama; Takaji Wakita; Naokazu Takeda; Tomoichiro Oka

Infectious acute gastroenteritis is an important public health problem worldwide. A total of 639 stool specimens were tested for the presence of diarrhea pathogens. The specimens were from outpatients with acute gastroenteritis who consulted the pediatric clinic in Kumamoto Prefecture, Japan, from June 2002 to December 2007. Of these, 421 (65.9%) were positive for diarrhea pathogens. Among them were norovirus (NoV) in 260 (61.8%), sapovirus (SaV) in 81 (19.2%), rotavirus in 49 (11.6%), adenovirus in 19 (4.5%), enterovirus in 13 (3.1%), astrovirus in 9 (2.1%), kobuvirus in 1 (0.2%), and bacterial pathogens in 11 (2.6%). Mixed infection (co‐infection of viruses) was found in 22 (5.2%) of the 421 pathogen‐positive stool samples. NoV was the most prevalent pathogen throughout the study period; however, the SaV detection rate was unexpectedly high and was found to be the secondary pathogen from 2005 to 2007. Genetic analysis of SaV with 81 strains demonstrated that SaV strains belonging to genogroup IV emerged in 2007, and dynamic genogroup changes occurred in a restricted geographic area. This study showed that SaV infection is not as rare as thought previously. J. Med. Virol. 81:1117–1127, 2009.


Archives of Virology | 2012

Human sapovirus classification based on complete capsid nucleotide sequences

Tomoichiro Oka; Kohji Mori; Nobuhiro Iritani; Seiya Harada; You Ueki; Setsuko Iizuka; Keiji Mise; Kosuke Murakami; Takaji Wakita; Kazuhiko Katayama

The genetically diverse sapoviruses (SaVs) are a significant cause of acute human gastroenteritis. Human SaV surveillance is becoming more critical, and a better understanding of the diversity and distribution of the viral genotypes is needed. In this study, we analyzed 106 complete human SaV capsid nucleotide sequences to provide a better understanding of their diversity. Based on those results, we propose a novel standardized classification scheme that meets the requirements of the International Calicivirus Scientific Committee. We believe the classification scheme and strains described here will be of value for the molecular characterization and classification of newly detected SaV genotypes and for comparing data worldwide.


Journal of Clinical Microbiology | 2011

Complete Genome Analysis of a Novel Intertypic Recombinant Human Adenovirus Causing Epidemic Keratoconjunctivitis in Japan

Hisatoshi Kaneko; Koki Aoki; Shigeaki Ohno; Hiroaki Ishiko; Tsuguto Fujimoto; Masayuki Kikuchi; Seiya Harada; Gabriel Gonzalez; Kanako O. Koyanagi; Hidemi Watanabe; Tatsuo Suzutani

ABSTRACT For 4 months from September 2008, 102 conjunctival swab specimens were collected for surveillance purposes from patients across Japan suspected of having epidemic keratoconjunctivitis (EKC). Human adenovirus (HAdV) DNA was detected in 61 samples by PCR, though the HAdV type for 6 of the PCR-positive samples could not be determined by phylogenetic analysis using a partial hexon gene sequence. Moreover, for 2 months from January 2009, HAdV strains with identical sequences were isolated from five conjunctival swab samples obtained from EKC patients in five different regions of Japan. For the analyses of the 11 samples mentioned above, we determined the nucleotide sequences of the entire penton base, hexon, and fiber genes and early 3 (E3) region, which are variable regions among HAdV types, and compared them to those of other HAdV species D strains. The nucleotide sequences of loops 1 and 2 in the hexons of all 11 samples showed high degrees of identity with those of the HAdV type 15 (HAdV-15) and HAdV-29 prototype strains. However, the fiber gene and E3 region sequences showed high degrees of identity with those of HAdV-9, and the penton base gene sequence showed a high degree of identity with the penton base gene sequences of HAdV-9 and -26. Moreover, the complete genome sequence of the 2307-S strain, which was isolated by viral culture from 1 of the 11 samples, was determined. The 2307-S strain was a recombinant HAdV between HAdV-9, -15, -26, -29, and/or another HAdV type; however, the recombination sites in the genome were not obvious. We propose that this virus is a novel intertypic recombinant, HAdV-15/29/H9, and may be an etiological agent of EKC.


Emerging Infectious Diseases | 2013

Human Gastroenteritis Outbreak Associated with Escherichia albertii, Japan

Tadasuke Ooka; Eisuke Tokuoka; Masato Furukawa; Tetsuya Nagamura; Yoshitoshi Ogura; Kokichi Arisawa; Seiya Harada; Tetsuya Hayashi

Although Escherichia albertii is an emerging intestinal pathogen, it has been associated only with sporadic human infections. In this study, we determined that a human gastroenteritis outbreak at a restaurant in Japan had E. albertii as the major causative agent.


Vaccine | 2010

Natural Japanese encephalitis virus infection among humans in west and east Japan shows the need to continue a vaccination program

Eiji Konishi; Yoko Kitai; Yukiko Tabei; Koichi Nishimura; Seiya Harada

Japanese encephalitis (JE) is a serious disease in Asia, but it can be prevented by vaccination. To evaluate the necessity for vaccination in areas with reduced numbers of vector mosquitoes, as well as patients, it is critical to understand the frequency of natural virus exposure. An antibody survey was recently conducted to estimate current natural infection rates in Japan, where the vaccination rate has dropped in recent years. Serum samples were collected in 2004-2008 from inhabitants of Kumamoto Prefecture in west Japan, and in 2004-2006 from the Tokyo Metropolitan area of east Japan. Average annual infection rates estimated from the prevalence of antibodies to the nonstructural 1 protein (NS1) of JE virus was 1.8% in Kumamoto and 1.3% in Tokyo. When estimated from percentages of populations with detectable neutralizing antibodies but with no vaccination history, the average annual infection rate was 2.6% in both survey areas. Thus, JE virus remains present and active in nature in Japan. Therefore, continuing a vaccination program is indispensable to prevent JE infection in humans.


Archives of Virology | 2012

A confirmation of sapovirus re-infection gastroenteritis cases with different genogroups and genetic shifts in the evolving sapovirus genotypes, 2002-2011

Seiya Harada; Tomoichiro Oka; Eisuke Tokuoka; Naoko Kiyota; Koichi Nishimura; Yasushi Shimada; Takehiko Ueno; Shigeru Ikezawa; Takaji Wakita; Qiuhong Wang; Linda J. Saif; Kazuhiko Katayama

Sapovirus (SaV) is an important pathogen that causes acute gastroenteritis in humans. Human SaV is highly diverse genetically and is classified into multiple genogroups and genotypes. At present, there is no clear evidence for gastroenteritis cases caused by re-infection with SaV. We found that two individuals were sequentially infected with SaVs of two different genogroups and had gastroenteritis after each infection, although in one of the subsequent cases, both SaV and norovirus were detected. We also found a genetic shift in SaVs from gastroenteritis outpatients in the same geographical location. Our results suggest that protective immunity may be at least genogroup-specific for SaV.


Genome Biology and Evolution | 2015

Defining the Genome Features of Escherichia albertii, an Emerging Enteropathogen Closely Related to Escherichia coli

Tadasuke Ooka; Yoshitoshi Ogura; Keisuke Katsura; Kazuko Seto; Hideki Kobayashi; Kimiko Kawano; Eisuke Tokuoka; Masato Furukawa; Seiya Harada; Shuji Yoshino; Junji Seto; Tetsuya Ikeda; Keiji Yamaguchi; Kazunori Murase; Yasuhiro Gotoh; Naoko Imuta; Junichiro Nishi; Tânia A. T. Gomes; Lothar Beutin; Tetsuya Hayashi

Escherichia albertii is a recently recognized close relative of Escherichia coli. This emerging enteropathogen possesses a type III secretion system (T3SS) encoded by the locus of enterocyte effacement, similar to enteropathogenic and enterohemorrhagic E. coli (EPEC and EHEC). Shiga toxin-producing strains have also been identified. The genomic features of E. albertii, particularly differences from other Escherichia species, have not yet been well clarified. Here, we sequenced the genome of 29 E. albertii strains (3 complete and 26 draft sequences) isolated from multiple sources and performed intraspecies and intragenus genomic comparisons. The sizes of the E. albertii genomes range from 4.5 to 5.1 Mb, smaller than those of E. coli strains. Intraspecies genomic comparisons identified five phylogroups of E. albertii. Intragenus genomic comparison revealed that the possible core genome of E. albertii comprises 3,250 genes, whereas that of the genus Escherichia comprises 1,345 genes. Our analysis further revealed several unique or notable genetic features of E. albertii, including those responsible for known biochemical features and virulence factors and a possibly active second T3SS known as ETT2 (E. coli T3SS 2) that is inactivated in E. coli. Although this organism has been observed to be nonmotile in vitro, genes for flagellar biosynthesis are fully conserved; chemotaxis-related genes have been selectively deleted. Based on these results, we have developed a nested polymerase chain reaction system to directly detect E. albertii. Our data define the genomic features of E. albertii and provide a valuable basis for future studies of this important emerging enteropathogen.


Open Forum Infectious Diseases | 2014

Phylogenetic Clades 6 and 8 of Enterohemorrhagic Escherichia coli O157:H7 With Particular stx Subtypes are More Frequently Found in Isolates From Hemolytic Uremic Syndrome Patients Than From Asymptomatic Carriers

Sunao Iyoda; Shannon D. Manning; Kazuko Seto; Keiko Kimata; Junko Isobe; Yoshiki Etoh; Sachiko Ichihara; Yuji Migita; Kikuyo Ogata; Mikiko Honda; Tsutomu Kubota; Kimiko Kawano; Kazutoshi Matsumoto; Jun Kudaka; Norio Asai; Junko Yabata; Kiyoshi Tominaga; Jun Terajima; Tomoko Morita-Ishihara; Hidemasa Izumiya; Yoshitoshi Ogura; Takehito Saitoh; Atsushi Iguchi; Hideki Kobayashi; Yukiko Hara-Kudo; Makoto Ohnishi; Reiko Arai; Masao Kawase; Yukiko Asano; Nanami Asoshima

EHEC O157:H7 clade 6 strains harboring stx2a and/or stx2c and clade 8 strains harboring stx2a or stx2a/stx2c were frequently associated with childhood HUS cases in Japan. Rapid and specific detection of such lineages are required for infection control measures.


Journal of Medical Virology | 2018

Recombinant type Human mastadenovirus D85 associated with epidemic keratoconjunctivitis since 2015 in Japan

Shintaro Hashimoto; Gabriel Gonzalez; Seiya Harada; Hideo Oosako; Nozomu Hanaoka; Rikutaro Hinokuma; Tsuguto Fujimoto

The aim of this study was to report the emergence of a recombinant human mastadenovirus (HAdV) type 85 (HAdV‐85) and to describe its genomic and clinical characteristics. The strains were detected and identified in Japan in cases of adenoviral conjunctivitis including epidemic keratoconjunctivitis (EKC). The type was designated as HAdV‐85 based on the novel combination of penton base (P = HAdV‐37), hexon (H = HAdV‐19), and fiber (F = HAdV‐8). The whole genome sequence determined for HAdV‐85 was compared against sequences of other types in the same species. The results of the phylogenetic analysis suggested a recombinant origin between HAdV‐53 and HAdV‐64, which have been two major causes of adenoviral EKC in Japan over the past decade. During the period between 2008 and 2016 in Kumamoto city, southwest of Japan, 311 cases diagnosed with conjunctivitis were diagnosed as being the consequence of adenoviral infections. Among them, 11 cases were determined to have been caused by HAdV‐85 since 2015. Thus, HAdV‐85 could be an emerging causative agent of adenoviral conjunctivitis.


Journal of Medical Virology | 2018

Broadly reactive real-time reverse transcription-polymerase chain reaction assay for detection of human sapovirus genotypes: OKA et al.

Tomoichiro Oka; Nobuhiro Iritani; Seiji Yamamoto; Kohji Mori; Tomoko Ogawa; Chika Tatsumi; Shinichiro Shibata; Seiya Harada; Fang-Tzy Wu

Sapoviruses are associated with acute gastroenteritis. Human sapoviruses are classified into four distinct genogroups (GI, GII, GIV, and GV) based on their capsid gene sequences. A TaqMan probe‐based real‐time reverse transcription‐polymerase chain reaction (RT‐PCR) assay that detects the representative strains of these four genogroups is widely used for screening fecal specimens, shellfish, and environmental water samples. However, since the development of this test, more genetically diverse sapovirus strains have been reported, which are not detectable by the previously established assays. In this study, we report the development of a broader‐range sapovirus real‐time RT‐PCR assay. The assay can detect 2.5 × 107 and 2.5 × 10 1 copies of sapovirus and therefore is as sensitive as the previous test. Analysis using clinical stool specimens or synthetic DNA revealed that the new system detected strains representative of all the 18 human sapovirus genotypes: GI.1‐7, GII.1‐8, GIV.1, and GV.1, 2. No cross‐reactivity was observed against other representative common enteric viruses (norovirus, rotavirus, astrovirus, and adenovirus). This new assay will be useful as an improved, broadly reactive, and specific screening tool for human sapoviruses.

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Tomoichiro Oka

National Institutes of Health

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Kazuhiko Katayama

National Institutes of Health

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Takaji Wakita

National Institutes of Health

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Hideki Kobayashi

National Agriculture and Food Research Organization

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