Detection of Human Parechoviruses from Clinical Stool Samples in Aichi, Japan

Between April 1999 and March 2008, a total of 4,976 stool specimens collected from patients with suspected viral infection through infectious agent surveillance in Aichi, Japan, were tested for the presence of human parechoviruses (HPeVs). We detected HPeVs in 110 samples by either cell culture, rev...

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Published inJournal of Clinical Microbiology Vol. 48; no. 8; pp. 2683 - 2688
Main Authors Ito, Miyabi, Yamashita, Teruo, Tsuzuki, Hideaki, Kabashima, Yuka, Hasegawa, Akiko, Nagaya, Satoko, Kawaguchi, Mariko, Kobayashi, Shinichi, Fujiura, Akira, Sakae, Kenji, Minagawa, Hiroko
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Published Washington, DC American Society for Microbiology 01.08.2010
American Society for Microbiology (ASM)
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Abstract Between April 1999 and March 2008, a total of 4,976 stool specimens collected from patients with suspected viral infection through infectious agent surveillance in Aichi, Japan, were tested for the presence of human parechoviruses (HPeVs). We detected HPeVs in 110 samples by either cell culture, reverse transcriptase PCR (RT-PCR), or both. Serotyping either by neutralization test or by nucleotide sequence determination and phylogenetic analysis of the VP1 region and 5' untranslated region (5'UTR) regions revealed that 63 were HPeV type 1 (HPeV-1), followed by 44 HPeV-3 strains, 2 HPeV-4 strains, and 1 HPeV-6 strain. The high nucleotide and amino acid sequence identities of the Japanese HPeV-3 isolates in 2006 to the strains previously reported from Canada and Netherlands confirmed the worldwide prevalence of HPeV-3 infection. Ninety-seven percent of the HPeV-positive patients were younger than 3 years, and 86.2% younger than 12 months. The clinical diagnoses of HPeV-positive patients were gastroenteritis, respiratory illness, febrile illness, exanthema, "hand, foot, and mouth disease," aseptic meningitis, and herpangina. Among 49 HPeV-positive patients with gastroenteritis, 35 were positive with HPeV-1 and 12 with HPeV-3, and out of 25 with respiratory illness, 11 were positive with HPeV-1 and 14 with HPeV-3. HPeV-3 seemed to be an important etiological agent of respiratory infection of children. While HPeV-1 was detected predominantly during fall and winter, the majority of the HPeV-3 cases were detected during summer and fall. A different pattern of clinical manifestations as well as seasonality suggested that there are different mechanisms of pathogenesis between HPeV-1 and HPeV-3 infections.
AbstractList Between April 1999 and March 2008, a total of 4,976 stool specimens collected from patients with suspected viral infection through infectious agent surveillance in Aichi, Japan, were tested for the presence of human parechoviruses (HPeVs). We detected HPeVs in 110 samples by either cell culture, reverse transcriptase PCR (RT-PCR), or both. Serotyping either by neutralization test or by nucleotide sequence determination and phylogenetic analysis of the VP1 region and 5' untranslated region (5'UTR) regions revealed that 63 were HPeV type 1 (HPeV-1), followed by 44 HPeV-3 strains, 2 HPeV-4 strains, and 1 HPeV-6 strain. The high nucleotide and amino acid sequence identities of the Japanese HPeV-3 isolates in 2006 to the strains previously reported from Canada and Netherlands confirmed the worldwide prevalence of HPeV-3 infection. Ninety-seven percent of the HPeV-positive patients were younger than 3 years, and 86.2% younger than 12 months. The clinical diagnoses of HPeV-positive patients were gastroenteritis, respiratory illness, febrile illness, exanthema, "hand, foot, and mouth disease," aseptic meningitis, and herpangina. Among 49 HPeV-positive patients with gastroenteritis, 35 were positive with HPeV-1 and 12 with HPeV-3, and out of 25 with respiratory illness, 11 were positive with HPeV-1 and 14 with HPeV-3. HPeV-3 seemed to be an important etiological agent of respiratory infection of children. While HPeV-1 was detected predominantly during fall and winter, the majority of the HPeV-3 cases were detected during summer and fall. A different pattern of clinical manifestations as well as seasonality suggested that there are different mechanisms of pathogenesis between HPeV-1 and HPeV-3 infections.
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Between April 1999 and March 2008, a total of 4,976 stool specimens collected from patients with suspected viral infection through infectious agent surveillance in Aichi, Japan, were tested for the presence of human parechoviruses (HPeVs). We detected HPeVs in 110 samples by either cell culture, reverse transcriptase PCR (RT-PCR), or both. Serotyping either by neutralization test or by nucleotide sequence determination and phylogenetic analysis of the VP1 region and 5' untranslated region (5'UTR) regions revealed that 63 were HPeV type 1 (HPeV-1), followed by 44 HPeV-3 strains, 2 HPeV-4 strains, and 1 HPeV-6 strain. The high nucleotide and amino acid sequence identities of the Japanese HPeV-3 isolates in 2006 to the strains previously reported from Canada and Netherlands confirmed the worldwide prevalence of HPeV-3 infection. Ninety-seven percent of the HPeV-positive patients were younger than 3 years, and 86.2% younger than 12 months. The clinical diagnoses of HPeV-positive patients were gastroenteritis, respiratory illness, febrile illness, exanthema, "hand, foot, and mouth disease," aseptic meningitis, and herpangina. Among 49 HPeV-positive patients with gastroenteritis, 35 were positive with HPeV-1 and 12 with HPeV-3, and out of 25 with respiratory illness, 11 were positive with HPeV-1 and 14 with HPeV-3. HPeV-3 seemed to be an important etiological agent of respiratory infection of children. While HPeV-1 was detected predominantly during fall and winter, the majority of the HPeV-3 cases were detected during summer and fall. A different pattern of clinical manifestations as well as seasonality suggested that there are different mechanisms of pathogenesis between HPeV-1 and HPeV-3 infections.Between April 1999 and March 2008, a total of 4,976 stool specimens collected from patients with suspected viral infection through infectious agent surveillance in Aichi, Japan, were tested for the presence of human parechoviruses (HPeVs). We detected HPeVs in 110 samples by either cell culture, reverse transcriptase PCR (RT-PCR), or both. Serotyping either by neutralization test or by nucleotide sequence determination and phylogenetic analysis of the VP1 region and 5' untranslated region (5'UTR) regions revealed that 63 were HPeV type 1 (HPeV-1), followed by 44 HPeV-3 strains, 2 HPeV-4 strains, and 1 HPeV-6 strain. The high nucleotide and amino acid sequence identities of the Japanese HPeV-3 isolates in 2006 to the strains previously reported from Canada and Netherlands confirmed the worldwide prevalence of HPeV-3 infection. Ninety-seven percent of the HPeV-positive patients were younger than 3 years, and 86.2% younger than 12 months. The clinical diagnoses of HPeV-positive patients were gastroenteritis, respiratory illness, febrile illness, exanthema, "hand, foot, and mouth disease," aseptic meningitis, and herpangina. Among 49 HPeV-positive patients with gastroenteritis, 35 were positive with HPeV-1 and 12 with HPeV-3, and out of 25 with respiratory illness, 11 were positive with HPeV-1 and 14 with HPeV-3. HPeV-3 seemed to be an important etiological agent of respiratory infection of children. While HPeV-1 was detected predominantly during fall and winter, the majority of the HPeV-3 cases were detected during summer and fall. A different pattern of clinical manifestations as well as seasonality suggested that there are different mechanisms of pathogenesis between HPeV-1 and HPeV-3 infections.
Author Yamashita, Teruo
Minagawa, Hiroko
Tsuzuki, Hideaki
Kabashima, Yuka
Fujiura, Akira
Kawaguchi, Mariko
Ito, Miyabi
Sakae, Kenji
Hasegawa, Akiko
Nagaya, Satoko
Kobayashi, Shinichi
AuthorAffiliation Department of Microbiology and Medical Zoology, Aichi Prefectural Institute of Public Health, Nagare 7-6, Tuji-machi, Kita-ku, Nagoya, Aichi 462-8576, Japan
AuthorAffiliation_xml – name: Department of Microbiology and Medical Zoology, Aichi Prefectural Institute of Public Health, Nagare 7-6, Tuji-machi, Kita-ku, Nagoya, Aichi 462-8576, Japan
Author_xml – sequence: 1
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  fullname: Yamashita, Teruo
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  fullname: Tsuzuki, Hideaki
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  fullname: Kabashima, Yuka
– sequence: 5
  fullname: Hasegawa, Akiko
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  fullname: Nagaya, Satoko
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  fullname: Kawaguchi, Mariko
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  fullname: Kobayashi, Shinichi
– sequence: 9
  fullname: Fujiura, Akira
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  fullname: Sakae, Kenji
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Snippet Between April 1999 and March 2008, a total of 4,976 stool specimens collected from patients with suspected viral infection through infectious agent...
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SubjectTerms 5' Untranslated Regions
Age Factors
Biological and medical sciences
Capsid Proteins - genetics
Cell Culture Techniques
Child, Preschool
Cluster Analysis
Feces - virology
Female
Fundamental and applied biological sciences. Psychology
Gastroenteritis - virology
Genotype
Humans
Infant
Infant, Newborn
Japan - epidemiology
Male
Microbiology
Miscellaneous
Molecular Sequence Data
Neutralization Tests
Parechovirus - growth & development
Parechovirus - isolation & purification
Picornaviridae Infections - diagnosis
Picornaviridae Infections - epidemiology
Picornaviridae Infections - pathology
Picornaviridae Infections - virology
Polymorphism, Genetic
Respiratory Tract Infections - virology
Reverse Transcriptase Polymerase Chain Reaction
RNA, Viral - genetics
Sequence Analysis, DNA
Sequence Homology
Serotyping
Virology
Virology - methods
Title Detection of Human Parechoviruses from Clinical Stool Samples in Aichi, Japan
URI http://jcm.asm.org/content/48/8/2683.abstract
https://www.ncbi.nlm.nih.gov/pubmed/20519478
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https://www.proquest.com/docview/754558923
https://www.proquest.com/docview/762268606
https://pubmed.ncbi.nlm.nih.gov/PMC2916555
Volume 48
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