Your search keyword '"Hiroaki Ishiko"' showing total 103 results

1. Macrolide Resistance–associated 23S rRNA Mutation in Mycoplasma genitalium, Japan

Author

Yasushi Shimada, Takashi Deguchi, Keita Nakane, Mitsuru Yasuda, Shigeaki Yokoi, Shin-ichi Ito, Masahiro Nakano, Shin Ito, and Hiroaki Ishiko

Subjects

bacteria, Mycoplasma genitalium, azithromycin, macrolide resistance, 23S rRNA, L4 ribosomal protein, Medicine, Infectious and parasitic diseases, RC109-216

Published

2011

2. Macrolide resistance--associated 23S rRNA mutation in mycoplasma genitalium, Japan

Author

Shimada, Yasushi, Deguchi, Takashi, Nakane, Keita, Yasuda, Mitsuru, Yokoi, Shigeaki, Ito, Shin-ichi, Nakano, Masahiro, Ito, Shin, and Hiroaki Ishiko

Subjects

Gene mutations -- Identification and classification, Macrolide antibiotics -- Dosage and administration, Drug resistance in microorganisms -- Genetic aspects, Mycoplasma genitalium -- Genetic aspects, Health

Abstract

To the Editor: Mycoplasma genitalium is now recognized as a serious pathogen in sexually transmitted infections (1,2). Azithromycin regimens have been commonly used for treatment of M. genitalium infections (3). [...]

Published

2011

3. Recombination analysis of intermediate human adenovirus type 53 in Japan by complete genome sequence

Author

Yoshifumi Ikeda, Hidemi Watanabe, Tatsuo Suzutani, Koki Aoki, Hiroaki Ishiko, Susumu Ishida, Shigeaki Ohno, Masako Nakamura, Nobuyoshi Kitaichi, Gabriel Gonzalez, Tsuguto Fujimoto, Kanako O. Koyanagi, and Hisatoshi Kaneko

Subjects

Recombination, Genetic, Whole genome sequencing, Genetics, Phylogenetic tree, Adenoviruses, Human, Molecular Sequence Data, Keratoconjunctivitis, Nucleic acid sequence, virus diseases, Genome, Viral, Sequence Analysis, DNA, Biology, Genome, Virology, eye diseases, Adenovirus Infections, Human, Japan, Phylogenetics, GenBank, Humans, Gene, Phylogeny, Recombination

Abstract

Human adenovirus type 53 (HAdV-53) has commonly been detected in samples from epidemic keratoconjunctivitis (EKC) patients in Japan since 1996. HAdV-53 is an intermediate virus, containing hexon-chimeric, penton base and fiber structures similar to HAdV-22 and -37, HAdV-37 and HAdV-8, respectively. HAdV-53-like intermediate strains were first isolated from EKC samples in Japan in the 1980s. Here, the complete genome sequences of three such HAdV-53-like intermediate strains (870006C, 880249C and 890357C) and four HAdV-53 strains were determined, and their relationships were analysed. The seven HAdV strains were classified into three groups, 870006C/880249C, 890357C and the four HAdV-53 strains, on the basis of phylogenetic analyses of the partial and complete genome sequences. HAdV strains within the same group showed the highest nucleotide identities (99.87–100.00 %). Like HAdV-53, the hexon loop 1 and 2 regions of 870006C, 880249C and 890357C showed the highest identity with HAdV-22. However, these strains did not show a hexon-chimeric structure similar to HAdV-22 and -37, or a penton base similar to HAdV-37. The fiber genes of 870006C and 880249C were identical to that of HAdV-37, but not HAdV-8. Thus, the three intermediate HAdVs isolated in the 1980s were similar to each other but not to HAdV-53. The recombination breakpoints were inferred by the Recombination Detection Program (rdp) using whole-genome sequences of these seven HAdV and of 12 HAdV-D strains from GenBank. HAdV-53 may have evolved from intermediate HAdVs circulating in the 1980s, and from HAdV-8, -22 and -37, by recombination of sections cut at the putative breakpoints.

Published

2011

4. Molecular Identification of Adenoviral Conjunctivitis in Turkey

Author

Sunay Duman, Tsunetada Konno, Server Yagci, Hiroaki Ishiko, Alper Akçali, Ramazan Yagci, and Etem Ozkaya

Subjects

Adult, 0106 biological sciences, 0301 basic medicine, Adolescent, Turkey, Acute Conjunctivitis, Viral Conjunctivitis, Polymerase Chain Reaction, 010603 evolutionary biology, 01 natural sciences, law.invention, Adenovirus Infections, Human, Diagnosis, Differential, Conjunctivitis, Viral, Young Adult, 03 medical and health sciences, law, Humans, Medicine, In patient, Typing, Cells, Cultured, Polymerase chain reaction, Retrospective Studies, Molecular identification, business.industry, Adenoviruses, Human, Incidence, Reproducibility of Results, General Medicine, Middle Aged, Isolation (microbiology), Virology, Ophthalmology, 030104 developmental biology, Cell culture, DNA, Viral, business, Conjunctiva

Abstract

Purpose. The aim of the study was isolation of adenoviruses by cell culture and identification using polymerase chain reaction (PCR) and phylogenetic analyses in patients clinically diagnosed with viral conjunctivitis in Ankara, Turkey. Methods. Conjunctival swabs from 34 patients with acute conjunctivitis were tested using cell culture isolation and PCR for adenovirus detection. PCR-positive samples were sequenced and typed. Results. The positive results of adenovirus were 26.5% (9 of 34) by the PCR method and 20.6% by culture isolation. Nine samples positive at PCR were identified by phylogenetic analyses as human adenovirus 8 (HAdV-8) (4 of 9), HAdV-3 (3 of 9), HAdV-4 (1 of 9), and HAdV-B (1 of 9). Conclusions. Our study showed types of adenoviruses in patients with ocular infection that occurred in this region of Turkey for the first time. Furthermore, sequence-based typing method is an efficient, accurate, and rapid means of diagnosis and typing of the adenovirus and has significant clinical and epidemiologic implications. HAdV-8 was major type for acute conjunctivitis in Ankara, Turkey. Further studies are required to reveal the major types of HAdVs that cause ocular diseases in this region of the world.

Published

2010

5. A comparison of the VP1, VP2, and VP4 regions for molecular typing of human enteroviruses

Author

Peter C. McMinn, Hiroyuki Shimizu, Phan Van Tu, Hiromu Yoshida, Mary Jane Cardosa, Hiroaki Ishiko, and David Perera

Subjects

Genetics, medicine.medical_specialty, Molecular epidemiology, viruses, Concordance, virus diseases, biochemical phenomena, metabolism, and nutrition, Biology, medicine.disease_cause, Virology, digestive system diseases, Infectious Diseases, Molecular genetics, Genotype, medicine, Enterovirus, Typing, Viral disease, Gene

Abstract

The VP4, VP2, and VP1 gene regions were evaluated for their usefulness in typing human enteroviruses. Three published RT-PCR primers sets targeting separately these three gene regions were used. Initially, from a total of 86 field isolates (36 HEV-A, 40 HEV-B, and 10 HEV-C) tested, 100% concordance in HEV-A was identified from all three gene regions (VP4, VP2, and VP1). However, for HEV-B and HEV-C viruses, only the VP2 and VP1 regions, and not VP4, showed 100% concordance in typing these viruses. To evaluate further the usefulness of VP4 in typing HEV-A enteroviruses, 55 Japanese and 203 published paired VP4 and VP1 nucleotide sequences were also examined. In each case, typing by VP4 was 100% in concordance with typing using VP1. Given these results, it is proposed that for HEV-A enteroviruses, all three gene regions (VP4, VP2, and VP1), would be useful for typing these viruses. These options would enhance the capability of laboratories in identifying these viruses and would greatly help in outbreaks of hand, foot, and mouth disease.

Published

2010

6. Analysis of the complete genome sequence of epidemic keratoconjunctivitis-related human adenovirus type 8, 19, 37 and a novel serotype

Author

Toshihide Ariga, Tatsuo Suzutani, Tomohiro Iida, Koki Aoki, Hisatoshi Kaneko, Takeshi Ohguchi, Shigeaki Ohno, Hiroaki Ishiko, and Yoshitsugu Tagawa

Subjects

Serotype, Molecular Sequence Data, Keratoconjunctivitis, Sequence Homology, Genome, Viral, Biology, Synteny, Genome, Adenovirus Infections, Human, Japan, Virology, Gene Order, Cluster Analysis, Humans, Phylogeny, Tropism, Genomic organization, Recombination, Genetic, Genetics, Whole genome sequencing, Phylogenetic tree, Adenoviruses, Human, virus diseases, Sequence Analysis, DNA, eye diseases, Hypervariable region, Epidemic Keratoconjunctivitis, DNA, Viral

Abstract

We determined the complete genome sequence of epidemic keratoconjunctivitis (EKC)-related human adenoviruses (HAdVs). We analysed a total of 12 HAdV strains; three prototype strains and two HAdV-8, three HAdV-19 and three HAdV-37 clinical isolates from EKC patients in Japan, and one novel serotype of HAdV. Genome organization of these serotypes was identical to those of the recently determined HAdV-19 and HAdV-37. The identities of the whole genome were over 99 % among strains from the same serotype, except for HAdV-19p, which is not associated with conjunctivitis, resulting in the formation of a distinct cluster in the phylogenetic analysis. The penton, loop 1 and loop 2 of hexon, early region 3 (E3) and fiber were hypervariable regions between serotypes. Results suggest that the HAdV-19 clinical strain is a recombinant of HAdV-19p-like and HAdV-37-like strains, and that the acquisition of the penton, E3 or fiber may be related to ocular tropism.

Published

2009

7. Nucleotide sequence variation in the hexon gene of human adenovirus type 8 and 37 strains from epidemic keratoconjunctivitis patients in Japan

Author

Takeshi Ohguchi, Tatsuo Suzutani, Koki Aoki, Hiroaki Ishiko, Yoshitsugu Tagawa, Shigeaki Ohno, and Hisatoshi Kaneko

Subjects

Molecular Sequence Data, Keratoconjunctivitis, Biology, medicine.disease_cause, Disease Outbreaks, Adenovirus Infections, Human, Japan, Virology, Genetic variation, medicine, Humans, Gene, Phylogeny, Genetics, Mutation, Base Sequence, Transition (genetics), Adenoviruses, Human, Nucleic acid sequence, Genetic Variation, virus diseases, medicine.disease, biology.organism_classification, eye diseases, Epidemic Keratoconjunctivitis, Mastadenovirus, Capsid Proteins

Abstract

Human adenovirus type 8 (HAdV-8) and 37 (HAdV-37) cause epidemic keratoconjunctivitis (EKC) associated with community-acquired and nosocomial infections. The nucleotide sequences of the entire hexon and fiber genes of eight HAdV-8 and 26 HAdV-37 strains were analysed and the transition mutations in each gene were compared among strains. Compared with prototype strains, the hexon gene of HAdV-8 and -37 strains showed between two and seven and one and twelve variations at nine and 21 different positions, respectively. All of these, except one position in HAdV-37, were located in the conserved region 4 (C4). There were only three polymorphisms in the fiber gene of both HAdV-8 and HAdV-37, fewer than those in C4. The nucleotide sequence of HAdV-8 and -37 C4 might be readily modified during EKC epidemics.

Published

2009

8. Novel Human Adenovirus Causing Nosocomial Epidemic Keratoconjunctivitis

Author

Shudo Yamazaki, Tsunetada Konno, Takeshi Ohguchi, Hiroaki Ishiko, Koki Aoki, Yoshitsugu Tagawa, Yasushi Shimada, Shigeaki Ohno, and Akio Hayashi

Subjects

Microbiology (medical), Serotype, Molecular Sequence Data, Keratoconjunctivitis, Virus, Disease Outbreaks, Microbiology, Adenovirus Infections, Human, Conjunctivitis, Viral, Japan, Phylogenetics, Virology, medicine, Humans, Phylogeny, Cross Infection, biology, Phylogenetic tree, Adenoviruses, Human, virus diseases, Sequence Analysis, DNA, medicine.disease, biology.organism_classification, eye diseases, Epidemic Keratoconjunctivitis, Mastadenovirus, Capsid Proteins, Viral disease

Abstract

In 2000, we encountered cases of nosocomial infections with epidemic keratoconjunctivitis (EKC) at a university hospital in Kobe, in the western part of Japan. Two human adenovirus (HAdV) strains, Kobe-H and Kobe-S, were isolated from patients with nosocomial EKC infection. They were untypeable by existing neutralizing antisera; however, the isolate was neutralized with homologous antisera. We then encountered several cases of EKC due to nosocomial infections in eye clinics in different parts of Japan. A total of 80 HAdVs were isolated from patients with EKC at eight different hospitals. The partial hexon gene sequences of the isolates were determined and compared to those of the prototype strains of 51 serotypes. All isolates had identical partial hexon nucleotide sequences. Phylogenetic analysis classified these isolates into species of HAdV-D. The isolates showed 93.9 to 96.7% nucleotide identity with HAdV-D prototype strains, while all 32 HAdV-D prototype strains ranged from 93.2 to 99.2% identity. The sequences of the loop 2 and fiber knob regions from the representative strain, Kobe-H, were dissimilar in all prototype strains of 51 serotypes. We believe that this virus is a novel serotype of HAdV that causes EKC.

Published

2008

9. Rapid Detection of the Mosaic Structure of the Neisseria gonorrhoeae penA Gene, Which Is Associated with Decreased Susceptibilities to Oral Cephalosporins

Author

Takashi Deguchi, Hiroaki Ishiko, Mitsuru Yasuda, and Susumu Ochiai

Subjects

DNA, Bacterial, Male, Microbiology (medical), medicine.drug_class, Sequence analysis, Molecular Sequence Data, Cephalosporin, Microbial Sensitivity Tests, medicine.disease_cause, Polymerase Chain Reaction, Sensitivity and Specificity, beta-Lactam Resistance, Bacterial genetics, Microbiology, Gonorrhea, Bacterial Proteins, polycyclic compounds, medicine, Humans, Penicillin-Binding Proteins, DNA Primers, Base Sequence, biology, Bacteriology, Sequence Analysis, DNA, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, Virology, Neisseria gonorrhoeae, Anti-Bacterial Agents, Cephalosporins, Neisseria cinerea, Neisseriaceae, Cefixime, Bacteria, medicine.drug

Abstract

In Neisseria gonorrhoeae , the mosaic structure of the penA gene (encoding penicillin-binding protein 2 [PBP 2]), which is composed of fragments of the penA genes from Neisseria cinerea and Neisseria perflava , has been significantly associated with decreased susceptibility to cephalosporins, particularly oral cephalosporins. The aim of this study was to develop a rapid assay for the detection of mosaic PBP 2 of N. gonorrhoeae by real-time PCR. This assay successfully detected the mosaic penA gene of N. gonorrhoeae , and its sensitivity was ≥10 1 copies/reaction. Six hundred twenty-one clinical strains were examined by this assay for the presence of mosaic PBP 2, which was detected in 85 (39.4%) of 216 strains from 2002, 69 (40.6%) of 170 strains from 2003, 71 (44.4%) of 160 strains from 2004, and 31 (41.3%) of 75 strains from 2005. The MICs of cephalosporins for strains with the mosaic PBP 2 detected by the assay were statistically higher than those for strains without the mosaic PBP 2. One hundred sixty-six (64.8%) of 256 strains with the mosaic PBP 2 exhibited cefixime MICs of ≥0.5 μg/ml. The emergence and spread of strains with mosaic PBP 2 could be a threat to the cefixime treatment of gonorrhea. This real-time PCR assay for the detection of mosaic PBP 2 of N. gonorrhoeae is thus useful in the prediction of decreased susceptibilities to oral cephalosporins.

Published

2008

10. Comparison of a Lateral-Flow Immunochromatography Assay with Real-Time Reverse Transcription-PCR for Detection of Human Metapneumovirus

Author

Hideaki Kikuta, Yutaka Takahashi, Nobuhisa Ishiguro, Yuichi Taguchi, Kunihiko Kobayashi, Reiko Gamo, Kazue Yasuda, Mutsuko Konno, Akio Hayashi, Chikako Sakata, Akihito Ishizaka, Yasutsugu Koga, Yoshinori Ogasawara, Hiroyuki Sawada, and Hiroaki Ishiko

Subjects

Male, Microbiology (medical), Time Factors, Paramyxoviridae, medicine.drug_class, viruses, Biology, Monoclonal antibody, Sensitivity and Specificity, Virus, Pneumovirinae, Human metapneumovirus, Nasopharynx, Virology, medicine, Humans, Metapneumovirus, Child, Mononegavirales, Respiratory Tract Infections, Chromatography, Paramyxoviridae Infections, Reverse Transcriptase Polymerase Chain Reaction, Antibodies, Monoclonal, Infant, Nucleocapsid Proteins, biology.organism_classification, Reverse transcription polymerase chain reaction, Child, Preschool, Female

Abstract

A lateral-flow immunochromatography (IC) assay for the detection of human metapneumovirus (hMPV) has been developed by using two mouse monoclonal antibodies to the nucleocapsid protein of hMPV. The purpose of this study was to compare the virus detection rate in nasopharyngeal secretions by the IC assay with that by real-time reverse transcription-PCR (RT-PCR). We collected nasopharyngeal swab samples from 247 children with respiratory symptoms in Sapporo, Japan, during the period from April to July 2007. Sixty-eight of the 247 children were positive for hMPV by real-time RT-PCR. When the real-time RT-PCR was used as the reference standard, the IC assay results were positive for 48 of the 68 real-time RT-PCR-positive children (70.6% sensitivity) and 8 of the 179 real-time RT-PCR-negative children (95.5% specificity). Although the sensitivity of the IC assay is lower than that of real-time RT-PCR, the IC assay is a rapid and useful test for the diagnosis of hMPV infections in children.

Published

2008

11. Molecular epidemiology of norovirus gastroenteritis in Soma, Japan, 2001–2003

Author

Mitsuaki Hosoya, Hitoshi Suzuki, Hiroaki Ishiko, Takashi Imamura, Yukihiko Kawasaki, Akio Hayashi, Osamu Hashimoto, Noriko Onishi, Masahiko Katayose, and Ayumi Matsumoto

Subjects

Pcr cloning, Genome, Viral, Biology, medicine.disease_cause, Microbiology, law.invention, fluids and secretions, Japan, law, medicine, Humans, Child, Polymerase chain reaction, Caliciviridae Infections, Molecular epidemiology, Phylogenetic tree, Reverse Transcriptase Polymerase Chain Reaction, Transmission (medicine), Norovirus, virus diseases, Outbreak, Virology, Gastroenteritis, Young age, Child, Preschool, Pediatrics, Perinatology and Child Health

Abstract

Background: The aim of the present paper was to investigate the molecular epidemiology of norovirus gastroenteritis in Japan using polymerase chain reaction (PCR) and subsequent phylogenetic analysis. Methods: From September 2001 to August 2003, 515 stool samples or rectal swabs were collected from almost all children visiting the Department of Pediatrics, Public Soma General Hospital with gastroenteritis. Samples were examined on reverse transcription (RT)-PCR to detect norovirus genome. The nucleotide sequences of the PCR products were determined and phylogenetic analysis performed. Results: The norovirus genome was detected in 66 samples. The peak season of norovirus gastroenteritis was from November 2001 to February 2002 and from September 2002 to December 2002. Norovirus gastroenteritis occurred most frequently in 1-year-old children. Norovirus strains produced four distinct clusters on phylogenetic analysis. Some strains detected in Soma were closely related to the strains detected in other regions in the world. The Mexico type and Lordsdale type were predominant in the 2001/2002 and 2002/2003 seasons, respectively, and the outbreaks continued for several months. Conclusions: Genetically different noroviruses might cause repeated gastroenteritis outbreaks every year in the Soma area. The long duration of the outbreak by a predominant strain in an epidemic season and the prevalence of infection mainly in the young age group suggested that norovirus epidemics were caused by person-to-person transmission rather than foodborne transmission. Based on molecular epidemiology, it is suggested that the annual prevalence of norovirus gastroenteritis in the Soma area might be caused by person-to-person transmission of genetically different norovirus strains, which might be transmitted from other region in the world.

Published

2008

12. Seroepidemiology of Human Bocavirus in Hokkaido Prefecture, Japan

Author

Tadashi Ariga, Hideaki Kikuta, Reza Shirkoohi, Xiaoming Ma, Rika Endo, Takashi Ebihara, Shinobu Teramoto, Nobuhisa Ishiguro, and Hiroaki Ishiko

Subjects

Microbiology (medical), Epidemiology, viruses, Blotting, Western, Fluorescent Antibody Technique, Spodoptera, Antibodies, Viral, Immunoglobulin G, Virus, Serology, Bocavirus, Parvoviridae Infections, Antibody Specificity, Seroepidemiologic Studies, Nasopharynx, Parvovirus B19, Human, Seroprevalence, Animals, 491.8, biology, Respiratory tract infections, Human bocavirus, biology.organism_classification, Virology, Titer, DNA, Viral, biology.protein, Antibody

Abstract

A new human virus, provisionally named human bocavirus (HBoV), was discovered by Swedish researchers in 2005. A new immunofluorescence assay using Trichoplusia ni insect cells infected with a recombinant baculovirus expressing the VP1 protein of HBoV was developed, and the levels of immunoglobulin G antibody to the VP1 protein of HBoV in serum samples were measured. The overall seroprevalence rate of antibodies against the VP1 protein of HBoV in a Japanese population aged from 0 months to 41 years was 71.1% (145 of 204). The seropositive rate was lowest in the age group of 6 to 8 months and gradually increased with age. All of the children had been exposed to HBoV by the age of 6 years. A rise in titers of antibody against the VP1 protein of HBoV during the convalescent phase was observed for four patients with lower respiratory tract infections, and HBoV DNA was detected in nasopharyngeal swab and serum samples from all four patients. These results suggest that HBoV is a ubiquitous virus acquired early in life and that HBoV might play a role in the course of lower respiratory tract infections.

Published

2007

13. The Herpes Simplex Virus Type 1 BgKLVariant, Unlike the BgOLVariant, Shows a Higher Association with Orolabial Infection than with Infections at Other Sites, Supporting the Variant-Dispersion-Replacement Hypothesis

Author

Rinji Kawana, Tomoo Itagaki, Toshiyuki Funabashi, Kamesaburo Yoshino, Hiroki Iga, Hiroshi Shiota, Takao Ikushima, Shigeru Yamamoto, Seiichiro Hata, Fumihiko Ban, Kozaburo Hayashi, Shunsaku Kobayashi, Hiroaki Ishiko, Shigeru Ozawa, Hiroyuki Eda, Yoshikazu Shimomura, Ryoichi Mori, Yoshikatsu Ozaki, Yasuyuki Ishii, Yoshio Numazaki, Tsuyoshi Sekizawa, Takeo Ogino, Kazuo Yanagi, and Takashi Nakakita

Subjects

Gene Expression Regulation, Viral, Microbiology (medical), Herpesvirus 1, Human, medicine.disease_cause, Herpesviridae, Virus, Cell Line, Conjunctivitis, Viral, Japan, Polymorphism (computer science), Virology, Alphaherpesvirinae, Genetic variation, medicine, Humans, BglII, Herpes Genitalis, biology, Genetic Variation, biology.organism_classification, Stomatitis, Herpetic, Herpes simplex virus, Keratitis, Herpetic, Herpes Labialis, Restriction fragment length polymorphism

Abstract

The identification and geographic distribution of the herpes simplex virus type 1 (HSV-1) BglII restriction fragment length polymorphism (RFLP) variants named BgKLand BgOLin clinical isolates from orolabial and cutaneous sites were described in our previous reports, in which the dispersion and replacement of HSV-1 variants were proposed. The base substitution sites deduced from the BgKLmultiple RFLP variations were mapped to the UL12 (DNase), RL2 (α0 transactivator), and latency-associated transcript genes in the present study. The results show that the relative frequencies (RFs) of BgKLare significantly higher in orolabial and cutaneous HSV-1 infections than in ocular infections. For the BgOLvariant, the opposite was found; i.e., the RF of BgOLwas significantly lower in orolabial and cutaneous infections than in ocular infections. No significant differences in the RFs of non-BgKL:non-BgOLisolates were observed. The ratio of the BgKLRF to the BgOLRF was much higher for the orolabial and cutaneous infection groups than for the ocular infection group, whereas the BgKLRF-to-non-BgKL:non-BgOLRF ratios for the former groups were slightly higher than those for the latter group. The higher efficiency of orolabial and cutaneous infections caused by BgKLcompared to the efficiency of infections caused by BgOLallows BgKLto spread more efficiently in human populations and to displace BgOL, because the mouth and lips are the most common HSV-1 infection sites in children. The present study supports our HSV-1 dispersion-and-replacement hypothesis and suggests that HSV-1, the latency-reactivation of which allows variants to accumulate in human populations, has evolved under competitive conditions, providing a new perspective on the polymorphism or variation of HSV-1.

Published

2007

14. Quantitative Detection of Ureaplasma parvum (biovar 1) and Ureaplasma urealyticum (biovar 2) in Urine Specimens from Men With and Without Urethritis by Real-Time Polymerase Chain Reaction

Author

Takashi Yoshida, Takashi Deguchi, Masayoshi Tamaki, Hiroaki Ishiko, Shin-Ichi Meda, Shigeaki Yokoi, Mitsuru Yasuda, and Yasuaki Kubota

Subjects

Male, Microbiology (medical), Sexually transmitted disease, Biovar, Mycoplasmataceae, Dermatology, Urinalysis, urologic and male genital diseases, medicine.disease_cause, Polymerase Chain Reaction, Ureaplasma, Microbiology, law.invention, fluids and secretions, Japan, Predictive Value of Tests, law, RNA, Ribosomal, 16S, medicine, Humans, Urethritis, Polymerase chain reaction, DNA Primers, biology, business.industry, Ureaplasma Infections, Public Health, Environmental and Occupational Health, bacterial infections and mycoses, medicine.disease, biology.organism_classification, female genital diseases and pregnancy complications, Infectious Diseases, Ureaplasma parvum, Mollicutes, bacteria, business, Ureaplasma urealyticum

Abstract

We previously reported a significant association between Ureaplasma urealyticum (biovar 2) and nongonococcal urethritis (NGU). We also found that the presence of Ureaplasma parvum (biovar 1) in the male urethra might be the result of colonization.The objective of this study was to clarify the pathogenic role of human Ureaplasma in NGU by assessing the association of bacterial loads with clinical findings and inflammatory responses in the urethra.The 16S rRNA gene of Ureaplasma was quantified by a TaqMan-based real-time polymerase chain reaction assay in first-pass urine from 37 men with Ureaplasma-positive nonmycoplasmal nonchlamydial NGU (NMNCNGU) and 30 Ureaplasma-positive men without urethritis.U. urealyticum (biovar 2) loads in 23 men with NMNCNGU were significantly higher than those in 14 men without urethritis. However, U. parvum (biovar 1) loads did not differ significantly between 14 men with NMNCNGU and 20 men without urethritis.The association of increased U. urealyticum (biovar 2) loads with symptomatic urethritis suggests that U. urealyticum (biovar 2) may be a pathogen of NGU. Our results also suggest that the presence of U. parvum (biovar 1) may not be significant in the development of NGU.

Published

2007

15. Decreased affinity of mosaic-structure recombinant penicillin-binding protein 2 for oral cephalosporins in Neisseria gonorrhoeae

Author

Takashi Deguchi, Mitsunobu Shimadzu, Satomi Sekiguchi, Hiroaki Ishiko, Mitsuru Yasuda, Osamu Kozawa, Rie Matsushima-Nishiwaki, Akio Hayashi, and Susumu Ochiai

Subjects

Male, Microbiology (medical), Sexually transmitted disease, Penicillin binding proteins, Administration, Oral, Spodoptera, Biology, medicine.disease_cause, Microbiology, Bacterial Proteins, polycyclic compounds, medicine, Animals, Humans, Penicillin-Binding Proteins, Pharmacology (medical), Cells, Cultured, Antibacterial agent, Pharmacology, Cephem, Mosaicism, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, Neisseria gonorrhoeae, Recombinant Proteins, Anti-Bacterial Agents, Cephalosporins, Penicillin, Neisseria cinerea, Infectious Diseases, bacteria, Neisseria, Baculoviridae, medicine.drug

Abstract

Objectives In Neisseria gonorrhoeae, the mosaic structure of penicillin-binding protein 2 (PBP 2), composed of fragments of PBP 2 from Neisseria cinerea and Neisseria perflava, was significantly associated with decreased susceptibility to cephalosporins, particularly oral cephalosporins. The aim of this study was to determine the affinity of mosaic PBP 2 for cephalosporins in N. gonorrhoeae. Methods Two types of non-mosaic PBP 2 from the type strain of N. gonorrhoeae (ATCC 19424) and a clinical strain (GU01-29), as well as the mosaic PBP 2 from a clinical strain (GU01-89), were expressed in insect cells, and recombinant PBP 2s were purified. ATCC 19424 and GU01-29 were susceptible to cephalosporins. GU01-89 showed decreased susceptibility to cephalosporins. Bindings of fluorescent penicillin to PBP 2 were characterized by the Scatchard plot analysis. The affinity of the recombinant PBP 2s for cefdinir, cefixime and ceftriaxone was determined by PBP 2 competition assays with fluorescent penicillin. Results The K(d) value of mosaic PBP 2 for fluorescent penicillin was higher than that of non-mosaic PBP 2s. The affinity of mosaic PBP 2 for cefdinir or cefixime was lower than that of the non-mosaic PBP 2s. The affinity of the mosaic PBP 2 for ceftriaxone was not changed, compared with that of the non-mosaic PBP 2s. Conclusions Other mechanisms may be involved in clinical isolates with decreased susceptibility to cephalosporins, but this study suggests that the decreased affinity of mosaic-structure recombinant PBP 2 for oral cephalosporins may contribute to decreased susceptibility to these antibiotics in N. gonorrhoeae.

Published

2007

16. Development of a Rapid Chromatographic Immunoassay for Detection of Human Metapneumovirus Using Monoclonal Antibodies Against Nucleoprotein of hMPV

Author

Takashi Ebihara, Nobuhisa Ishiguro, Susumu Ochiai, Reiko Gamo, Hiroaki Ishiko, Takashi Sato, Chikako Sakata, Hideaki Kikuta, and Rika Endo

Subjects

medicine.drug_class, viruses, Immunology, Monoclonal antibody, Genome, Cell Line, Viral Proteins, Human metapneumovirus, Transcription (biology), medicine, Animals, Humans, Immunology and Allergy, Immunoassay, Chromatography, Paramyxoviridae Infections, biology, medicine.diagnostic_test, Structural protein, Antibodies, Monoclonal, virus diseases, RNA, biology.organism_classification, Macaca mulatta, Virology, respiratory tract diseases, Nucleoprotein, Nucleoproteins, Metapneumovirus

Abstract

Human metapneumovirus (hMPV) nucleocapsid (N) protein is a major structural protein that encapsidates the RNA genome and is essential for replication and transcription of the hMPV genome. We developed two mouse monoclonal antibodies (MAbs), designated 3D1 and 5B10, against N protein of hMPV and characterized them by an immunofluorescence assay and an immunoprecipitation assay using Trichoplusia ni (Tn5) insect cells infected with a recombinant baculovirus-expressing hMPV N protein. Both MAbs were found to be reactive to two groups of hMPV by an immunofluorescence assay using two groups of hMPV-infected cells. A chromatographic immunoassay (lateral flow assay) was developed using the MAbs. The assay is a sandwich immunoassay that uses a paper membrane with a gold colloid-conjugated MAb (5B10) in a liquid phase and an MAb (3D1) in a solid phase. We preliminarily examined the sensitivity and specificity using hMPV-infected cells, Tn5 insect cells infected with a recombinant baculovirus-expressing hMPV N protein, hMPV, and purified N protein. The assay had good specificity and sufficient sensitivity to detect hMPV. Therefore, the assay may be a rapid and useful test for diagnosis of hMPV infections.

Published

2007

17. Anti-adenoviral effect of anti-HIV agents in vitro in serotypes inducing keratoconjunctivitis

Author

Shigeaki Ohno, Hiroaki Ishiko, Eiichi Uchio, Kazuaki Kadonosono, Aki Fuchigami, Koki Aoki, and Akio Hayashi

Subjects

Virus Cultivation, Nevirapine, Anti-HIV Agents, Gene Dosage, Biology, Cell Line, Adenovirus Infections, Human, Conjunctivitis, Viral, Cellular and Molecular Neuroscience, Amprenavir, Zalcitabine, chemistry.chemical_compound, Indinavir, medicine, Humans, Reverse-transcriptase inhibitor, Reverse Transcriptase Polymerase Chain Reaction, Adenoviruses, Human, Stavudine, Epithelial Cells, medicine.disease, Virology, Sensory Systems, Ophthalmology, chemistry, DNA, Viral, Adenoviral keratoconjunctivitis, medicine.drug, Cidofovir

Abstract

Around one million people are affected by adenoviral keratoconjunctivitis a year in Japan, and it is recognized as one of the major pathogens of ophthalmological nosocomial infection worldwide. Although cidofovir can be used systemically for immunocompromised patients with disseminated adenoviral infection, no specific anti-adenoviral agent has been established for the treatment of adenoviral infection. We evaluated the anti-adenoviral effect of anti-HIV (human immunodeficiency virus) agents in this study. Five anti-HIV agents (zalcitabine, stavudine, nevirapine, indinavir and amprenavir) were subjected to in vitro evaluation. A549 cells were used for viral cell culture, and adenovirus serotypes 3, 4, 8, 19 and 37 were used. After calculating CC50 (50% cytotoxic concentration) of each agent by MTS (3-(4,5-dimethylthiazol-2-yl)-5-(3-carboxymethoxyphenyl)-2-(4-sulfophenyl)-2H-tetrazolium) method, we cultured adenovirus with the agents for seven days and quantitatively measured extracted adenoviral DNA by real-time PCR. Among the anti-HIV drugs, zalcitabine and stavudine, both nucleoside reverse transcriptase inhibitors, showed significant anti-adenoviral activity. In contrast, nevirapine, a non-nucleoside reverse transcriptase inhibitor, and indinavir and amprenavir, which are both protease inhibitors, were ineffective against adenovirus. These results indicate that zalcitabine and stavudine are possible candidates for the local and systemic treatment of adenoviral infection, and the anti-adenoviral effect might depend on the pharmacological properties of anti-HIV agents. The chemical properties on the clinical safety for systemic and local application need to be determined in order to for these drugs to be accepted for the treatment of adenovirus in clinical settings.

Published

2007

18. Antiadenoviral Effect of the α5β1 Integrin Receptor Ligand, GRGDSP Peptide, in Serotypes That Cause Acute Keratoconjunctivitis

Author

Kazuaki Kadonosono, Hiroaki Ishiko, Ryoji Kimura, Aya Fuchigami, Eiichi Uchio, Koki Aoki, Akio Hayashi, Shigeaki Ohno, and Yuh-Huey Huang

Subjects

Serotype, Adenoviridae Infections, Integrin, Keratoconjunctivitis, Peptide, Biology, Ligands, Virus Replication, medicine.disease_cause, Antiviral Agents, Virus, Adenoviridae, Cell Line, medicine, Humans, Serotyping, Receptor, chemistry.chemical_classification, Dose-Response Relationship, Drug, General Medicine, Ligand (biochemistry), medicine.disease, Virology, Sensory Systems, Ophthalmology, chemistry, Acute Disease, biology.protein, Oligopeptides, Integrin alpha5beta1

Abstract

Background/Aims: In adenoviral conjunctivitis, the infection process starts by the attachment of adenoviral fibers to conjunctival epithelial cells that contain the receptor for the adenovirus. The α5β1 integrin receptor ligand, GRGDSP peptide, contains the arginine-glycine-aspartate-binding motif which is common to the Coxsackie adenovirus receptor and integrins that are known to be adenoviral receptors. We evaluated the antiadenoviral effect of an expected adenoviral receptor inhibitor, GRGDSP peptide,in vitro. Methods: Adenovirus types 3, 4, 8, 19 and 37 were used. After calculating the 50% cytotoxic concentration of GRGDSP peptide, the adenovirus was cultivated with the agent for 7 days under serial dilution. Adenoviral DNA was qualitatively measured by real-time PCR. Results: GRGDSP peptide showed an inhibitory effect against adenoviral proliferation in all serotypes except type 4 in a dose-dependent manner. Conclusion: This result suggests that the α5β1 integrin receptor ligand, GRGDSP peptide, has antiadenoviral activity in vitro, and the possibility of being used for local treatment of epidemic keratoconjunctivitis.

Published

2007

19. Detection of antibodies against human metapneumovirus by western blot using recombinant nucleocapsid and matrix proteins

Author

Takashi Ebihara, Rika Endo, Hideaki Kikuta, Nobuhisa Ishiguro, Eri Kawai, Hiroaki Ishiko, and Xiaoming Ma

Subjects

Adult, Adolescent, Myeloma protein, viruses, Blotting, Western, Biology, Antibodies, Viral, Immunofluorescence, law.invention, Viral Matrix Proteins, Human metapneumovirus, Antigen, Western blot, law, Virology, medicine, Humans, Child, medicine.diagnostic_test, Infant, virus diseases, Nucleocapsid Proteins, biology.organism_classification, Molecular biology, respiratory tract diseases, Titer, Infectious Diseases, Child, Preschool, Recombinant DNA, biology.protein, Metapneumovirus, Antibody

Abstract

Detection of antibodies against individual proteins of human metapneumovirus (hMPV) is important in the analysis of immune responses to hMPV. Specific antibodies against nucleocapsid (N) and matrix (M) proteins in 97 serum samples were tested by Western blot using recombinant N and M proteins of hMPV expressed in Escherichia coli. The results were compared with those of immunofluorescence assays (IFAs) based on hMPV-infected LLC-MK2 cells, which expressed the whole hMPV proteins. Thirty (61.2%) and 31 (63.3%) of 49 serum samples with titers of >/=1:160 by IFA reacted with N and M proteins, respectively. Only 2 (4.2%) of 11 serum samples with titers of 1:80 by IFA reacted with N and M proteins. Antibodies against N and M proteins were not detected in 37 serum samples with titers of

Published

2006

20. Production and Characterization of Neutralizing Monoclonal Antibodies Against Human Metapneumovirus F Protein

Author

Xiaoming Ma, Rika Endo, Takashi Ebihara, Hiroaki Ishiko, Nobuhisa Ishiguro, and Hideaki Kikuta

Subjects

medicine.drug_class, viruses, Viral pathogenesis, Immunology, Fluorescent Antibody Technique, Immunofluorescence, Monoclonal antibody, Polymerase Chain Reaction, Neutralization, Epitope, Cell Line, Viral Proteins, Human metapneumovirus, Neutralization Tests, medicine, Animals, Immunology and Allergy, Metapneumovirus, biology, medicine.diagnostic_test, Antibodies, Monoclonal, virus diseases, biology.organism_classification, Macaca mulatta, Virology, respiratory tract diseases, biology.protein, Antibody

Abstract

Human metapneumovirus (hMPV) F protein promotes fusion of viral and cell membranes, and is thought to be a major antigenic determinant that mediates effective neutralization and protection against hMPV infection. In this paper, the development of two mouse monoclonal antibodies (MAbs) by immunization with hMPVinfected cells is described. Immunofluorescence assay (IFA) using hMPV F protein-expressing cells indicated that two MAbs, designated 1G3 and 9B10, recognized hMPV F protein. Both MAbs were found to be reactive to two groups of hMPV by an IFA using two groups of hMPV-infected cells. The 9B10 mAb had strong neutralizing activity against both groups of hMPV, while the 1G3 MAb had only weak neutralization activity. These results indicate that the hMPV F protein is a major antigenic determinant that mediates extensive cross-lineage neutralization and protection. Production of MAbs to the hMPV F protein is critical for development of diagnostic techniques, vaccine research, and studies on viral pathogenesis.

Published

2005

21. Polymerase Chain Reaction-Based Subtyping of Ureaplasma Parvum and Ureaplasma Urealyticum in First-Pass Urine Samples from Men With or Without Urethritis

Author

Hiroaki Ishiko, Yasuaki Kubota, Takashi Deguchi, Takashi Yoshida, Mitsuru Yasuda, Yuri Nomura, Masayoshi Tamaki, Yoshito Takahashi, and Shin-ichi Maeda

Subjects

DNA, Bacterial, Male, Microbiology (medical), Serotype, Genotype, Dermatology, urologic and male genital diseases, medicine.disease_cause, Polymerase Chain Reaction, Ureaplasma, law.invention, Microbiology, fluids and secretions, Species Specificity, law, medicine, Humans, Urethritis, Polymerase chain reaction, business.industry, Ureaplasma Infections, Public Health, Environmental and Occupational Health, Mycoplasma, bacterial infections and mycoses, medicine.disease, female genital diseases and pregnancy complications, Subtyping, Infectious Diseases, Ureaplasma parvum, bacteria, business, Chlamydia trachomatis, Ureaplasma urealyticum

Abstract

Background: Our previous study suggested a significant association between Ureaplasma urealyticum and nongonococcal urethritis (NGU). However, association of the serovars of U. urealyticum with NGU remains unclear. A polymerase chain reaction (PCR)-based assay can distinguish 4 serovars of Ureaplasma parvum from each other and categorize 10 serovars of U. urealyticum into 3 subtypes: subtype 1 (serovars 2, 5, 8, and 9), subtype 2 (serovars 4, 10, 12, and 13), and subtype 3 (serovars 7 and 11). Goal: The goal of this study was to determine which subtypes of U. urealyticum are associated with NGU as determined by PCR-based assay. Study: The prevalence of U. urealyticum subtypes in 106 ureaplasma-positive men with urethritis was compared with that in 30 ureaplasma-positive men without urethritis. Results: In men with nonchlamydial NGU and men with Mycoplasma genitalium-negative nonchlamydial NGU, only U. urealyticum subtype 1 (serovars 2, 5, 8, and 9) was detected significantly more often than in men without urethritis. Conclusion: This study suggests that subtype 1 of U. urealyticum (serovars 2, 5, 8, and 9) is associated with NGU independently of Chlamydia trachomatis or M. genitalium.

Published

2005

22. Phylogenetic analysis of wild-type 1 polioviruses isolated during the final period of transmission in Turkey

Author

Cigdem Artuk, Kikuko Miyamura, Shudo Yamazaki, Etem Ozkaya, Rika Miura, Yasushi Shimada, Iffet Alaeddinoglu, and Hiroaki Ishiko

Subjects

Time Factors, Turkey, viruses, Biology, medicine.disease_cause, World health, law.invention, Viral Proteins, Phylogenetics, law, Virology, medicine, Humans, Phylogeny, Phylogenetic tree, Poliovirus, Wild type, medicine.disease, Poliomyelitis, Cysteine Endopeptidases, Transmission (mechanics), Period (geology), Capsid Proteins

Abstract

The last poliomyelitis case associated with a wild poliovirus in Turkey occurred in November 1998. This was the last known case of paralytic poliomyelitis caused by indigenous wild poliovirus in the World Health Organization's European Region. This study investigated the genetic relationships of wild-type 1 polioviruses at the latest period of transmission. A phylogenetic tree was constructed on the basis of the VP1/2A sequence from 14 wild-type 1 polioviruses isolated from Turkey in 1994–1998, along with those from other areas of the world. The Turkey isolates in the latest period of transmission were closely related to each other, forming a cluster distinct from other strains. The results showed that these viruses had been spreading indigenously in the eastern and south-eastern parts of Turkey, and ceased transmission there during 1998. This finding serves as a reference for future poliovirus surveillance both in Turkey and worldwide.

Published

2004

23. Association of Ureaplasma urealyticum (Biovar 2) With Nongonococcal Urethritis

Author

Takashi Yoshida, Mitsuru Yasuda, Takashi Deguchi, Takamaro Miyazawa, Masayoshi Tamaki, Shin-ichi Maeda, and Hiroaki Ishiko

Subjects

Adult, Male, Microbiology (medical), Adolescent, Biovar, Chlamydia trachomatis, Dermatology, medicine.disease_cause, Microbiology, Japan, Prevalence, medicine, Humans, Urethritis, Aged, biology, business.industry, Ureaplasma Infections, Public Health, Environmental and Occupational Health, Chlamydia Infections, Middle Aged, biology.organism_classification, medicine.disease, Infectious Diseases, Ureaplasma parvum, Case-Control Studies, business, Ureaplasma urealyticum

Abstract

The tiny (T)-strain mycoplasmas, designated in 1974 as Ureaplasma urealyticum, have been divided into 2 species, Ureaplasma parvum (biovar 1) and U. urealyticum (biovar 2), but association of each of these species with nongonococcal urethritis (NGU) remains unclear.The goal of this study was to determine whether U. parvum (biovar 1) or U. urealyticum (biovar 2) is associated with NGU.The prevalences of U. parvum (biovar 1) and U. urealyticum (biovar 2) in 572 patients with urethritis were compared with those in 141 men without urethritis.The prevalence of U. urealyticum (biovar 2) in men with NGU (15.8%) or with nonchlamydial NGU (18.0%) was significantly higher than that in men without urethritis (7.8%). The prevalence of U. parvum (biovar 1) in men with NGU (8.5%) or with nonchlamydial NGU (11.1%) did not differ significantly from that in men without urethritis (13.5%).Our results showed a significant association between U. urealyticum (biovar 2) and NGU. They also suggest that the presence of U. parvum (biovar 1) in the male urethra might be the result of colonization.

Published

2004

24. Human Metapneumovirus Infection in Japanese Children

Author

Yutaka Takahashi, Hideaki Kikuta, Nobuhisa Ishiguro, Kunihiko Kobayashi, Takashi Ebihara, Hiroaki Ishiko, Michimaru Hara, and Rika Endo

Subjects

Male, Microbiology (medical), Adolescent, viruses, Biology, Antibodies, Viral, Immunoglobulin G, Serology, Human metapneumovirus, Virology, medicine, Humans, Metapneumovirus, Child, Phylogeny, Paramyxoviridae Infections, Reverse Transcriptase Polymerase Chain Reaction, Infant, Newborn, Infant, virus diseases, medicine.disease, biology.organism_classification, respiratory tract diseases, Pneumonia, Upper respiratory tract infection, Immunoglobulin M, Child, Preschool, Immunology, biology.protein, Bronchitis, Female

Abstract

Human metapneumovirus (hMPV) has been recently discovered as an etiological agent of acute respiratory infections. Our purpose was to asses the virological and clinical features of children with respiratory infections caused by hMPV. We examined 658 nasopharyngeal swab samples obtained from 637 children with respiratory infections for hMPV by using reverse transcription-PCR (RT-PCR). A total of 268 samples from 637 children were inoculated onto tertiary monkey kidney cells. A total of 36 serum samples (26 in the acute phase and 10 in the convalescent phase) from the 26 hMPV-positive children were tested for immunoglobulin G (IgG) and IgM antibodies to hMPV by using an indirect immunofluorescence assay. We detected hMPV in 57 (8.9%) of the 637 samples by using RT-PCR and isolated 7 (2.6%) hMPV strains of the 268 samples in cell cultures. A total of 12 (46.2%) of 26 hMPV-positive children were suspected to have primary infection with hMPV as determined by an indirect immunofluorescence assay. The infected children were diagnosed as having wheezy bronchitis (36.8%), upper respiratory tract infection (26.3%), bronchitis (22.8%), and pneumonia (14.0%). We showed that two hMPV groups were circulating in different regions during the same period and that reinfection with hMPV frequently occurs in childhood. The RT-PCR test is the most sensitive test for detection of hMPV, and a serological test may be useful to differentiate between primary infection and reinfection with hMPV.

Published

2004

25. Cytokine-dependent anti-viral role of CD4-positive T cells in therapeutic vaccination against chronic hepatitis B viral infection

Author

Kiwamu Okita, Yuhki Yamaguchi, Hiroaki Ishiko, Keiko Korenaga, Keisuke Hino, Takahiro Yamasaki, Akio Hayashi, Kiyomi Funatsuki, Fenyu Ren, Muneko Furutani, Tomomi Konishi, and Satoyoshi Yamashita

Subjects

Adult, CD4-Positive T-Lymphocytes, Male, Hepatitis B virus, medicine.medical_treatment, T cell, Lymphocyte Activation, medicine.disease_cause, Interferon-gamma, Hepatitis B, Chronic, Antigen, Virology, Humans, Cytotoxic T cell, Medicine, Hepatitis B Vaccines, Prospective Studies, Aged, Hepatitis B Surface Antigens, Tumor Necrosis Factor-alpha, business.industry, ELISPOT, Immunotherapy, Active, Middle Aged, Vaccination, Treatment Outcome, Infectious Diseases, Cytokine, medicine.anatomical_structure, Immunology, Cytokines, Female, business, CD8

Abstract

There are several lines of evidence suggesting that specific vaccine therapy with a standard hepatitis B virus (HBV) vaccination reduces HBV replication. The aim of this study was to investigate the anti-viral mechanism of vaccine therapy in chronic hepatitis B patients. Nineteen patients were assigned to receive either vaccine therapy (n = 13) or no treatment as a control (n = 6). Vaccinated patients were analyzed for T cell proliferative responses specific for envelope antigen and cytokine production by antigen-specific T cells. ELISPOT and cytotoxicity assays also were carried out for limited blood samples. Serum HBV DNA levels decreased significantly at 3 months after completion of therapy and thereafter as compared to the baseline ones, and were significantly lower in vaccinated patients than in controls at 12 and 18 months after completion of therapy. Vaccination induced antigen-specific CD4+ T cell proliferative responses in four patients (30.8%). The production of high levels of interferon-γ (IFN-γ) and tumor necrosis factor-α (TNF-α) by antigen-specific T cells was found in six patients (46.0%) who showed significantly lower HBV DNA levels in serum at 6 (P = 0.04) and 18 months (P = 0.005) after completion of therapy than those without high levels of cytokine production. Vaccination did not induce antigen-specific CD8+ T cells or cytotoxic T cells. These results suggest that envelope-specific CD4+ T cells may control directly HBV replication by producing anti-viral cytokines rather than providing help for cytotoxic T cells in therapeutic vaccination against chronic HBV infection. J. Med. Virol. 71:376–384, 2003. © 2003 Wiley-Liss, Inc.

Published

2003

26. Production and release of infectious hepatitis C virus from human liver cell cultures in the three-dimensional radial-flow bioreactor

Author

Yoshiharu Matsuura, Seishi Nagamori, Mami Matsuda, Tomokazu Matsuura, Masaaki Kawada, Hayato Kawakami, Hideki Aizaki, Osamu Hashimoto, Satoshi Hasumura, Hiroaki Ishiko, Tetsuro Suzuki, and Tatsuo Miyamura

Subjects

Infectious clone, Hepatitis C virus, In vitro culture model, Replication, medicine.disease_cause, Serial passage, Virology, medicine, Artificial liver, Full-length cDNA, Polymerase, Three-dimensional radial-flow bioreactor, Infectivity, biology, virus diseases, RNA, digestive system diseases, NS2-3 protease, Particles, Viral replication, Reverse genetics, Cell culture, HCV, biology.protein, Infection

Abstract

Lack of efficient culture systems for hepatitis C virus (HCV) has been a major obstacle in HCV research. Human liver cells grown in a three-dimensional radial-flow bioreactor were successfully infected following inoculation with plasma from an HCV carrier. Subsequent detection of increased HCV RNA suggested viral replication. Furthermore, transfection of HCV RNA transcribed from full-length cDNA also resulted in the production and release of HCV virions into supernatant. Infectivity was shown by successful secondary passage to a new culture. Introduction of mutations in RNA helicase and polymerase regions of HCV cDNA abolished virus replication, indicating that reverse genetics of this system is possible. The ability to replicate and detect the extracellular release of HCV might provide clues with regard to the persistent nature of HCV infection. It will also accelerate research into the pathogenicity of HCV, as well as the development of prophylactic agents and new therapy.

Published

2003

27. Sequence Analysis of Pephd Within Hcv E2 Region and Correlation With Resistance of Interferon Therapy in Japanese Patients Infected With Hcv Genotypes 2A and 2B

Author

Takeshi Saito, Mari Yonaha, Akio Miyokawa, Keiji Mitamura, Kenichi Morikawa, Takayoshi Ito, and Hiroaki Ishiko

Subjects

Adult, Male, Genotype, Sequence analysis, medicine.medical_treatment, Hepatitis C virus, Eukaryotic Initiation Factor-2, Hepacivirus, Biology, medicine.disease_cause, Antiviral Agents, eIF-2 Kinase, Japan, Viral Envelope Proteins, Sequence Analysis, Protein, Interferon, Drug Resistance, Viral, medicine, Humans, Amino Acid Sequence, NS5A, Conserved Sequence, Aged, Sequence Homology, Amino Acid, Hepatology, Gastroenterology, virus diseases, Middle Aged, Hepatitis C, Protein kinase R, Virology, digestive system diseases, Cytokine, Mutation, Immunology, Female, Interferons, Viral disease, Hepatitis C Antigens, medicine.drug

Abstract

Objective Hepatitis C virus (HCV) E2 protein was recently reported to have a double-stranded RNA-activated protein kinase–eukaryotic initiation factor 2α (PKR-eIF2α) phosphorylation homology domain (PePHD); PKR is induced by interferon (IFN). PePHD interacts with PKR and inactivates it. PePHD could be a predictor for IFN response, like the interferon sensitivity determination region (ISDR) of HCV NS5A. Several groups reported that PePHD is conserved, and mutations in this region do not correlate with IFN response. In this study, we further investigated the amino acid variation of PePHD among four major genotypes and its correlation with IFN response. Methods We enrolled 74 patients for this study and determined PePHD sequence of HCV derived from sera of patients infected with HCV genotype 1a (1 patient; nonresponder [NR]), 1b (36 patients; 4 complete responders [CR], 32 NR), 2a (29 patients; 17 CR, 12 NR), and 2b (8 patients; 3 CR, 5 NR). We also analyzed mutations in ISDR of HCV genotype 1b in 31 patients. Results PePHD had several variations among four genotypes investigated. In patients infected with HCV genotype 1b, PePHD sequence was well conserved and seemed to have no correlation with IFN response. Mutations in ISDR were correlated with IFN response. In patients with HCV genotypes 2a and 2b, PePHD had multiple variations, and one particular motif, “RGQQ-” at the N-terminus, showed a close correlation with IFN resistance. All eight patients with HCV containing this motif were IFN nonresponders. Conclusions IFN resistance of HCV correlates with its “RGQQ-” motif at the N-terminus of PePHD in HCV genotype 2a and 2b. PePHD of HCV could be a predictor of IFN resistance in patients infected with HCV genotype 2a and 2b.

Published

2003

28. Rapid Detection of Mycoplasma genitalium , Mycoplasma hominis , Ureaplasma parvum , and Ureaplasma urealyticum Organisms in Genitourinary Samples by PCR-Microtiter Plate Hybridization Assay

Author

Takashi Deguchi, Shin-ichi Maeda, Takashi Yoshida, Takamaro Miyazawa, and Hiroaki Ishiko

Subjects

Microbiology (medical), biology, Ureaplasma infection, Mycoplasmataceae, Mycoplasma, Mycoplasma hominis, urologic and male genital diseases, biology.organism_classification, medicine.disease_cause, medicine.disease, Virology, female genital diseases and pregnancy complications, Microbiology, Ureaplasma, Ureaplasma parvum, medicine, Mycoplasma genitalium, Ureaplasma urealyticum

Abstract

We present a method for detecting the presence of Mycoplasma genitalium , Mycoplasma hominis , Ureaplasma parvum , and Ureaplasma urealyticum organisms, which are thought to be associated with nongonococcal urethritis (NGU) and other genitourinary infections, in clinical samples. This method consists of PCR amplification of a part of the 16S rRNA gene followed by 96-well microtiter plate hybridization assay using four species-specific capture probes to detect the targets. To test the efficacy of this method, we applied it to the detection of the four species in the urine of patients with NGU. There were no cross-reactions with other human mycoplasmas or ureaplasmas, and the PCR-microtiter plate hybridization assay detected as few as 10 copies of the 16S rRNA gene of each of the four species. Based on these results, this PCR-microtiter plate hybridization assay can be considered an effective tool for the diagnosis of genitourinary infections with mycoplasmas or ureaplasmas.

Published

2003

29. TT virus infection during childhood

Author

Hitoshi Ohto, Niro Ujiie, Chikako Takeuchi, Akira Sato, Akio Hayashi, Hiroaki Ishiko, Tsutomu Nishizawa, and Hiroaki Okamoto For The Vertical Transmission of He

Subjects

Adult, Male, Genotype, Immunology, Population, Mothers, Physiology, Comorbidity, Hepacivirus, Biology, Virus, law.invention, Pregnancy, Seroepidemiologic Studies, law, Humans, Immunology and Allergy, Risk factor, education, Polymerase chain reaction, Torque teno virus, education.field_of_study, Liver Diseases, Infant, Newborn, Infant, Sequence Analysis, DNA, Hematology, Viral Load, DNA Virus Infections, Infectious Disease Transmission, Vertical, Child, Preschool, Cord blood, DNA, Viral, RNA, Viral, Female, Viral disease, Viral load

Abstract

BACKGROUND: TT virus (TTV) is widespread in the general population, however, the mode of its transmission and the mechanism of maintaining it in the general population are unclear. STUDY DESIGN AND METHODS: To determine the possible mother-to-infant route of transmission, 54 infants born to 50 anti-HCV-positive mothers were assessed longitudinally. Nucleotide sequences amplified by seminested PCR with primers targeting the N22 variable coding region of genotypes 1 through 6 were compared in mothers and their infants. RESULTS: The prevalence of TTV DNA was 30 percent (15/50; 95% CI, 18-45) in mothers and 44 percent (24/54; 95% CI, 31-59) in their infants. TTV DNA was detected during a follow-up period in 13 (87%; 95% CI, 60–98) of 15 infants born to infected mothers and in 11 (28%; 95% CI, 15-45) of 39 infants born to DNA-negative mothers. None of 38 cord blood samples, but one of 14 blood samples, obtained at 1 month of age had detectable TTV DNA. The lowest infection rate at the earliest ages and the subsequent increasing prevalence of infection (22% at 6 months and 33%[43% cumulative rate] at 2 years) is consistent with an age-dependent acquisition of TTV by nonparenteral routes. In 13–mother-infant pairs positive for TTV DNA, six showed a high degree of nucleotide sequence similarity (99.1-100%), whereas the remaining seven pairs differed more than 10 percent from each other (46.8-89.2%). The viral load of maternal blood was not a plausible risk factor for transmission. Genotype 1, of which pathogenicity failed to be shown by measurement of hepatic enzymes, was more rapidly cleared (88 vs. 8% other genotypes, p < 0.001) among infants. CONCLUSIONS: These observations strongly suggest that the main factor for TTV acquisition in children involves their age-associated increase in environmental interactions with infectious materials. Genotype 1 might be involved in a weak or a limited pathologic role, which can possibly be diluted by other harmless genotypes.

Published

2002

30. Macrolide Resistance–associated 23S rRNA Mutation inMycoplasma genitalium, Japan

Author

Shin Ito, Yasushi Shimada, Shinichi Ito, Mitsuru Yasuda, Takashi Deguchi, Shigeaki Yokoi, Masahiro Nakano, Keita Nakane, and Hiroaki Ishiko

Subjects

Ribosomal Proteins, Microbiology (medical), macrolide resistance, Epidemiology, letter, lcsh:Medicine, Mycoplasma genitalium, Biology, urologic and male genital diseases, medicine.disease_cause, Azithromycin, lcsh:Infectious and parasitic diseases, Microbiology, Antibiotic resistance, Japan, 23S ribosomal RNA, Ribosomal protein, Drug Resistance, Bacterial, medicine, Humans, Mycoplasma Infections, lcsh:RC109-216, Letters to the Editor, bacteria, Escherichia coli, Gene, Pathogen, Retrospective Studies, azithromycin, L22 ribosomal protein, Urethritis, lcsh:R, 23S rRNA, bacterial infections and mycoses, biology.organism_classification, Virology, female genital diseases and pregnancy complications, Anti-Bacterial Agents, RNA, Ribosomal, 23S, Infectious Diseases, Mutation, Macrolides, L4 ribosomal protein, medicine.drug

Abstract

To the Editor: Mycoplasma genitalium is now recognized as a serious pathogen in sexually transmitted infections (1,2). Azithromycin regimens have been commonly used for treatment of M. genitalium infections (3). However, failure of azithromycin treatment has been reported in cases of M. genitalium–positive nongonococcal urethritis (NGU) (4,5), and macrolide-resistant strains of M. genitalium have been isolated from case-patients in Australia, Sweden, and Norway for whom azithromycin treatment has failed (4,5). In these strains, mutations in the 23S rRNA gene were associated with macrolide resistance, and mutations in ribosomal protein genes L4 and L22 were also found (5). Surveillance for antimicrobial resistance of M. genitalium is essential to identify antimicrobial resistant strains and to then determine appropriate treatment. Coculture of patient specimens with Vero cells has improved the primary isolation rate of M. genitalium from clinical specimens and offered some current clinical strains for antimicrobial drug susceptibility testing (6). To determine their antimicrobial susceptibilities, a molecular real-time PCR method has been developed (7,8). However, isolating M. genitalium from clinical specimens and antimicrobial drug susceptibility testing of clinical isolates remain labor-intensive, time-consuming tasks. In addition, no methods are available to directly determine antimicrobial drug susceptibilities of M. genitalium in clinical specimens. To monitor macrolide susceptibilities in clinical strains of M. genitalium in Japan, therefore, we examined M. genitalium DNA found in the urine of men with NGU for the presence of macrolide resistance–associated mutations in the 23S rRNA gene and the ribosomal protein genes L4 and L22. This retrospective study was approved by the Institutional Review Board of the Graduate School of Medicine, Gifu University, Gifu, Japan. We collected pretreatment urine specimens from 308 men with NGU who had visited a urologic clinic (iClinic) in Sendai, Japan, during 2006 through 2008 and stored the specimens at –70°C. Each man gave informed consent. Twenty-five of 58 urine specimens confirmed to be positive for M. genitalium by PCR-based assay were randomly chosen for this study and subjected to DNA purification. The 23S rRNA gene and the ribosomal proteins genes L4 and L22 of M. genitalium were amplified from the purified DNA by PCR as reported previously and then sequenced (5). In 1 specimen, we found an A-to-G transition at nucleotide position 2072 in the 23S rRNA gene of M. genitalium, corresponding to position 2059 in Escherichia coli (Table). An A2059 (E. coli numbering) residue in region V of the 23S rRNA gene is critical for the binding of macrolides (9). Mutations of A2058, A2059, and other 23S rRNA residues within the macrolide-binding site can confer a high-level resistance to macrolides in several bacterial species, including M. genitalium (5,9). Therefore, M. genitalium strains that harbor the A2059G (E. coli numbering) mutation in the 23S rRNA gene could be highly macrolide resistant. We also found a T-to-G transition at nucleotide position 2199 in the 23S rRNA gene of M. genitalium, corresponding to position 2185 in E. coli, in 3 specimens, but this mutation has not been associated with macrolide resistance in other bacterial species (9). Table Mutations in the 23S rRNA gene and amino acid changes in L4 and L22 ribosomal proteins of 25 Mycoplasma genitalium strains in the pretreatment urine specimens of men with nongonococcal urethritis, Japan We found amino acid changes in L4 and L22 ribosomal proteins in M. genitalium in 9 specimens. L4 and L22 ribosomal proteins each have extended loops, which converge to form a narrowing in the exit tunnel adjacent to the macrolide-binding site (10). Therefore, macrolide resistance–associated missense mutations in L4 and L22 tend to be localized to Gln62–Gly66 in L4 and Arg88-Ala93 in L22 of E. coli, which are closest to the macrolide-binding site (10). All of the amino acid changes in L4 of M. genitalium found in this study corresponded to those at the downstream regions from Gln62-Gly66 in L4 of E. coli. Of the amino acid changes in L22 of M. genitalium, the only Gly93Glu change found in M. genitalium harboring the A2059G (E. coli numbering) mutation in the 23S rRNA gene was located within the region corresponding to Arg88-Ala93 in L22 of E. coli. In this strain, therefore, the Gly93Glu change in L22 might contribute to the increase of macrolide resistance. The patient with NGU, whose specimen exhibited this strain of M. genitalium that harbored both the A2059G (E. coli numbering) mutation in the 23S rRNA gene and in which the Gly93Glu change in L22 was detected, was given a single dose of 1 g azithromycin and was clinically cured of NGU. However, the present study suggests that M. genitalium strains with high-level macrolide resistance might have already emerged in clinical settings in Japan. The emergence and spread of such a clinical mutant could threaten the ability of macrolides to treat M. genitalium infections. We should continue monitoring macrolide resistance of M. genitalium clinical strains. The nonculture approach used in our study will be useful until culturing of mycoplasmas from clinical specimens and antimicrobial drug susceptibility testing can be performed easily in laboratories.

Published

2011

31. Heterogeneous, restricted patterns of Epstein–Barr virus (EBV) latent gene expression in patients with chronic active EBV infection

Author

Mikio Yoshioka, Nobuhisa Ishiguro, Hideaki Kikuta, Kunihiko Kobayashi, Xiaoming Ma, and Hiroaki Ishiko

Subjects

Adult, Male, Epstein-Barr Virus Infections, Herpesvirus 4, Human, Adolescent, viruses, Biology, medicine.disease_cause, Genome, Virus, Viral Matrix Proteins, Viral Proteins, Chronic active EBV infection, hemic and lymphatic diseases, Virology, Gene expression, otorhinolaryngologic diseases, medicine, Humans, In patient, RNA, Messenger, Child, Gene, Reverse Transcriptase Polymerase Chain Reaction, medicine.disease, Epstein–Barr virus, BZLF1, DNA-Binding Proteins, stomatognathic diseases, Epstein-Barr Virus Nuclear Antigens, Child, Preschool, Chronic Disease, Immunology, Trans-Activators, RNA, Viral, Female

Abstract

Epstein–Barr virus (EBV) has been shown to infect T lymphocytes and to be associated with a chronic active infection (CAEBV), which has been recognized as a mainly non-neoplastic T-cell lymphoproliferative disorder (T-cell LPD). The systemic distribution of EBV genomes was studied, by real-time PCR, in multiple tissues from six patients with CAEBV, including three patients with T-cell LPD, one patient with B-cell LPD and two patients with undetermined cell-type LPD. There were extremely high loads of EBV genomes in all tissues from the patients. This reflects an abundance of circulating and infiltrating EBV-infected cells and a wide variety of clinical symptoms in the affected tissues. We chose one sample from each patient that was shown by real-time PCR to contain a high load of EBV genomes and examined the expression of EBV latent genes by RT–PCR. EBER1 and EBNA1 transcripts were detected in all samples. Only one sample also expressed EBNA2, LMP1 and LMP2A transcripts in addition to EBER1 and EBNA1 transcripts. Two of the remaining five samples expressed LMP1 and LMP2A transcripts. One sample expressed LMP2A but not LMP1 and EBNA2 transcripts. Another sample expressed EBNA2 but not LMP1 and LMP2A transcripts. The other sample did not express transcripts of any of the other EBNAs or LMPs. None of the samples expressed the viral immediate-early gene BZLF1. These results showed that EBV latent gene expression in CAEBV is heterogeneous and that restricted forms of EBV latency might play a pathogenic role in the development of CAEBV.

Published

2001

32. Genetic analysis of recent Taiwanese isolates of a variant of coxsackievirus A24

Author

Cheng-Hsien Chang, Seigo Yamamoto, Min-Muh Sheu, Hiroaki Ishiko, Kuei-Hsiang Lin, Naokazu Takeda, Yaowapa Pongsuwanna, Wen-Loong Huang, Pei-Yu Chu, Chi-Liang Chern, Heng-Lin Wang, and Syuji Yoshino

Subjects

Time Factors, Genotype, Taiwan, Coxsackievirus Infections, Sequence alignment, Biology, medicine.disease_cause, Genetic analysis, Evolution, Molecular, Cytopathogenic Effect, Viral, Phylogenetics, Virology, medicine, Humans, Point Mutation, Amino Acid Sequence, Codon, Base Pairing, Phylogeny, Enterovirus, Genetics, Genetic diversity, Base Sequence, Sequence Homology, Amino Acid, Reverse Transcriptase Polymerase Chain Reaction, Nucleic acid sequence, Acute hemorrhagic conjunctivitis, medicine.disease, Infectious Diseases, Amino Acid Substitution, RNA, Viral, Conjunctivitis, Acute Hemorrhagic, Sequence Alignment

Abstract

Epidemics of acute hemorrhagic conjunctivitis (AHC) caused by a variant of coxsackievirus A24 (CA24v) reappeared in Taiwan in 1990 and 1994, following the first two epidemics of 1985--86 and 1988--89. To analyze the genetic diversity of recent CA24v in Taiwan, 7 Taiwanese strains isolated during the 1990--94 period were studied together with one Japanese and two Thai strains isolated in 1993. A fragment of 674 nucleotides between the carboxy terminal 3A and the amino terminal 3D polymerase, including the entire 3C protease (3C(pro)), was amplified by a reverse transcription-polymerase chain reaction (RT-PCR) and the nucleotide sequences were determined. In the 549 nucleotides (183 amino acids) of the entire 3C(pro), we found nucleotide differences at 80 positions between 10 strains and the prototype strain, EH24/70, one of the earliest strains of CA24v. Most of the nucleotide changes were synonymous substitutions and only nine amino acid changes were found. The nucleotide sequence homologies among 71 strains worldwide were 88-100%. These 71 nucleotide sequences were then analyzed by Neighbor-joining method and phylogenetically separated into three distinct genotypes. Genotype I consisted of early strains isolated in 1970--71 from Singapore and Hong Kong. Genotype II included isolates from Singapore and Thailand obtained in 1975. Genotype III comprised strains from the eastern hemisphere isolated in 1985--94 from Japan, Taiwan, China, Hong Kong, Thailand, Singapore, Pakistan and Ghana. They were further divided chronologically into six clusters. The recent isolates from Taiwan obtained in 1985/1986, 1988/1989 and 1990--94 were classified into genotype III Clusters 1, 5, and 6 respectively. The evolutionary rate was re-estimated to be 3 x 10(- 3) 30 years after the emergence of the virus.

Published

2001

33. Analysis of plasma viral RNA levels during acute dengue virus infection using quantitative competitor reverse transcription-polymerase chain reaction

Author

Ananda Nisalak, Jaroslav Zivny, Hiroaki Ishiko, Francis A. Ennis, Joyce E. Norman, David W. Vaughn, T. Mirawati Sudiro, Sharone Green, Siripen Kalayanarooj, and Alan L. Rothman

Subjects

biology, RNA, Dengue virus, biology.organism_classification, medicine.disease, medicine.disease_cause, Virology, Virus, Dengue fever, Flavivirus, Infectious Diseases, Viral replication, medicine, Viral disease, Viral load

Abstract

There is increasing recognition of the potential importance of viral burden in the pathogenesis of dengue hemorrhagic fever (DHF). There is little data available, however, describing the kinetics of viral replication in humans with natural dengue virus (DV) infection. Standard procedures for measuring titers of infectious virus in clinical specimens are either laborious or insensitive. We developed a method for measurement of DV RNA in plasma samples based on reverse transcription-polymerase chain reaction (RT-PCR) using a mutant RNA target as a competitor. This technique was reproducible and accurate for samples containing any of the four DV serotypes, and could be applied to samples containing as few as 250 copies of RNA per reaction. We examined plasma viral RNA levels in 80 children with acute DV infection; sequential plasma samples were tested in 34 of these children. Plasma viral RNA levels ranged as high as 109 RNA copies/ml, and correlated with titers of infectious virus measured in mosquitoes (r = 0.69). Plasma viral RNA levels fell rapidly during the last several days of the febrile period. We did not find a significant difference in maximal plasma viral RNA levels between children with DHF and children with dengue fever, but peak viral RNA levels were identified in only 16 subjects. We conclude that this quantitative RT-PCR method will be valuable for further studies of natural DV infections. J. Med. Virol. 63:29–34, 2001. © 2001 Wiley-Liss, Inc.

Published

2000

34. Outbreak of severe neurologic involvement associated with enterovirus 71 infection

Author

Hiroshi Takada, Yoshitaka Shimizu, Hiroshi Komatsu, Hiroaki Ishiko, and Yoshihiro Takeuchi

Subjects

Male, Pediatrics, medicine.medical_specialty, Pathology, Antibodies, Viral, medicine.disease_cause, Herpangina, Disease Outbreaks, Central nervous system disease, Central Nervous System Infections, Japan, Developmental Neuroscience, Enterovirus Infections, medicine, Enterovirus 71, Humans, Child, Enterovirus, biology, Reverse Transcriptase Polymerase Chain Reaction, business.industry, Infant, Newborn, Infant, Outbreak, Aseptic meningitis, medicine.disease, biology.organism_classification, Blotting, Southern, Neurology, Child, Preschool, Pediatrics, Perinatology and Child Health, RNA, Viral, Female, Neurology (clinical), business, Meningitis, Encephalitis

Abstract

Enterovirus 71 has been associated with several outbreaks, as well as sporadic cases, of central nervous system infection and has a worldwide distribution. Seven children with encephalitis and five with aseptic meningitis caused by Enterovirus 71 were seen at Otsu Municipal Hospital during the summer of 1997. The infections were confirmed serologically, although detection of the viral genome in cerebrospinal fluid was unsuccessful. Seven children were diagnosed as having hand-foot-and-mouth syndrome, two were diagnosed as having herpangina, and three patients younger than 12 months old developed no eruptions. The skin or mucosal manifestations of this outbreak demonstrated considerable variation. The Enterovirus 71 strain that caused the outbreak had a strong neurovirulent tendency. Among the patients with encephalitis, symptoms originating from the impairment of diencephalon were seen in four patients, and those originating from cerebellar impairment were seen in two patients. Brain magnetic resonance imaging in one patient revealed an abnormality in the pons. The neurologic manifestations associated with Enterovirus 71 infection may be characterized by involvement of the cerebellum, brainstem, and diencephalon. Enterovirus 71 is one of the pathogenic viruses that cause hand-foot-and-mouth syndrome, as well as a variety of other clinical manifestations. The most important of these is neurologic disease, especially in infants and young children.

Published

1999

35. Microplate-reverse hybridization method to determine dengue virus serotype

Author

T. Mirawati Sudiro, Siripen Kalayanarooj, Ananda Nisalak, Sharone Green, Hiroaki Ishiko, Francis A. Ennis, David W. Vaughn, Diana E Kershaw, and Alan L. Rothman

Subjects

Dengue virus, medicine.disease_cause, Sensitivity and Specificity, Virus, law.invention, Dengue fever, Dengue, law, Ethidium, Virology, medicine, Humans, Serotyping, Polymerase chain reaction, Staining and Labeling, biology, Reverse Transcriptase Polymerase Chain Reaction, Hybridization probe, Dengue Virus, biology.organism_classification, medicine.disease, Molecular biology, Reverse transcriptase, Flavivirus, Real-time polymerase chain reaction, RNA, Viral

Abstract

A reverse transcriptase-polymerase chain reaction (RT-PCR) and microplate-reverse hybridization method were developed to detect and type dengue viruses in patients plasma specimens. A silica method was used to isolate RNA; and 3'-noncoding region universal primers were used to amplify dengue virus RNA. Using RT-PCR and ethidium bromide staining we could detect dengue virus in serum spiked with serially diluted dengue virus with a level of sensitivity similar to that of a quantitative fluorescent focus assay of dengue viruses in cell culture, i.e. 1.4 fluorescent focus units per reaction. Applying this assay to 14 dengue-positive plasma samples and 13 dengue-negative samples, dengue viremia was detectable by RT-PCR with a sensitivity comparable to mosquito inoculation. To determine the serotypes, digoxigenin-labeled PCR products from plasma samples and six laboratory adapted dengue viruses were hybridized in stringent conditions to serotype-specific DNA probes immobilized on microplates, and the hybridized product was detected with a colorimetric assay. Serotypes of dengue viruses, in cell culture and in patient plasma specimens, were identified using this method.

Published

1998

36. Molecular Epidemiology of Adenoviral Conjunctivitis in Hanoi, Vietnam

Author

Takeshi Ohguchi, Shigeaki Ohno, Hiroaki Ishiko, Xue-Hai Jin, Nguyen Thanh Ha, Koki Aoki, and Masataka Akanuma

Subjects

Serotype, Pcr cloning, Polymerase Chain Reaction, law.invention, Adenovirus Infections, Human, Conjunctivitis, Viral, law, conjunctivitis, Humans, Medicine, Polymerase chain reaction, Chromatography, Molecular Epidemiology, Molecular epidemiology, business.industry, Adenoviruses, Human, Nucleic acid sequence, virus diseases, adenovirus, Virology, eye diseases, Ophthalmology, Real-time polymerase chain reaction, Vietnam, Clinical diagnosis, DNA, Viral, Immunologic Techniques, real-time PCR, business, Conjunctiva

Abstract

Purpose To investigate the serotypes of adenovirus causing conjunctivitis in Hanoi, Vietnam. Design Clinical diagnosis of adenoviral conjunctivitis and laboratory-based experimental study. Methods We collected 21 conjunctival swabs from 21 different patients with a clinical presentation compatible with adenoviral conjunctivitis, in Hanoi, Vietnam. Immunochromatography and real-time polymerase chain reaction (PCR) were performed to detect human adenovirus (HAdV). The sequence of PCR products was analyzed to determine the serotype of HAdV. Results Of 21 samples, HAdV DNA was detected in 14 samples (66.7%) by real-time PCR. The serotype analysis showed HAdV-8 in 11 samples (78.6%), HAdV-3 in two samples (14.3%), and HAdV-37 in one sample (7.1%). Of 11 HAdV-8 samples, one sample (9.1%) was prototype, and the other 10 samples (90.9%) had identical nucleotide sequence and were identified as a variant of HAdV-8. Conclusions HAdV-8 was found to be the predominant serotype in Hanoi, Vietnam. Most of the HAdV-8 samples were a variant of HAdV-8.

Published

2006

37. Serotype Determination of Enteroviruses That Cause Hand-foot-mouth Disease

Author

Hiroaki Ishiko, Tadaomi Tokutake, Akio Hayashi, Kenji Sakae, Narisawa Tadashi, Naokazu Takeda, Yutaka Minohara, Yoshihisa Ashihara, Tatsuo Kato, and Akiko Kitamura

Subjects

Serotype, biology, viruses, General Medicine, biology.organism_classification, medicine.disease_cause, Virology, Neutralization, Virus, Blot, Enterovirus 71, medicine, Enterovirus, Peptide sequence, Southern blot

Abstract

Coxsackievirus A16 (CA16) and enterovirus 71 (EV71) are known to be major causative agents of hand-foot-and-mouth disease prevalent in summer in Japan. Discrimination and identification of these viruses were often hampered by a nonneutralizable or nontypable virus. Therefore, a Southern blot hybridization that utilizes mixed probes specific to serotype was developed. Firstly, an approximately 650 bases spanning 5'-noncoding region to one third of VP2 including entire VP4 was amplified with a set of primers containing enterovirus common sequences and a genomic RNA as template. Secondary, the nucleotide sequences were determined using seven CA16 and eighteen EV71 strains including the standard strains, and the deduced amino acid sequences of VP4 were searched to find residues which are conserved in the same serotypes but diverged among different serotypes. Candidate positions for the mixed probes were defined at the carboxyl terminus of VP4. Thirdly, Southern blot analyses were carried out using thirty-nine enterovirus standard strains, seven CA16 isolates and sixty-six EV71 isolates previously identified by the neutralization test. The results revealed that each mixed probe exclusively bound to the homologous DNAs but not to the heterologous ones. In an attempt to determine serotypes without virus isolation, clinical specimens from hand-foot-and-mouth disease were examined. Of 78 throat swabs and 15 vesicular fluids, 71 (91.0%) and 13 (86.7%) specimens were clearly identified, indicating that the method described here offer advantages over the traditional neutralization assay: It is rapid, specific and less labor-consuming.

Published

1997

38. The incidence of viremia and the heterogeneity of hepatitis C Virus genotypes among blood donors, hemophiliacs and patients with chronic liver disease

Author

T.C. Aw, Naokazu Takeda, Osamu Hashimoto, Ponnudurai Kuperan, and Hiroaki Ishiko

Subjects

Adult, Male, Adolescent, Genotype, Hepatitis C virus, Blood Donors, Viremia, Hepacivirus, Hemophilia A, medicine.disease_cause, Chronic liver disease, Virus, Pathology and Forensic Medicine, Flaviviridae, medicine, Humans, Retrospective Studies, Hepatitis, biology, business.industry, Liver Diseases, Incidence (epidemiology), virus diseases, Alanine Transaminase, Middle Aged, medicine.disease, biology.organism_classification, Chronic Disease, Immunology, Female, Viral disease, business

Abstract

Hepatitis C Virus (HCV) is the major cause of parentally transmitted non-A, non-B hepatitis. We studied the incidence of HCV Viremia in blood donors, hemophiliacs and patients with chronic liver disease who are positive for antibodies to HCV, and then correlated the HCV genotypes among the three groups. 23 blood donors, 10 hemophiliacs and 97 patients with chronic liver disease were found to be positive for anti-HCV during this study period from June 1993 to December 1993. Only 3 (13%) blood donors, 6 (60%) hemophiliacs and 71 (73%) patients with chronic liver disease were found to be viremic when tested for HCV RNA by reverse transcriptase-polymerase chain reaction (RT-PCR). The low incidence of viremia among blood donors may be due to any one of the following three reasons. 1, the level of viremia was below the level of detection. 2, the viremia was intermittent with persistent infection. 3, the majority of cases represented resolved infection. The HCV genotypes were heterogeneous among the three groups. All the blood donors with viremia and 35 (50%) of patients with chronic liver disease, belonged to type II (1b). However only one (17%) of the hemophiliacs belonged to type II (1b). Studies have shown that the genotype I(1a) is the predominant type in the USA and Europe, whereas type II(1b) is more frequent in the Far East. It is also suggested that type II (1b) is associated with non-responsiveness to interferon therapy. Our hemophiliacs were treated with imported coagulation factors, thus they were probably exposed to the genotypes in the west. There was significant difference in the incidence of HCV type II (1b) among local blood donors and hemophiliacs (P = 0.005). However the difference between the hemophiliacs and the patients with chronic liver disease was not statistically significant. The number of patients in this study was too small to draw any firm conclusions. However the findings highlight the importance of studying the genotypes of patients with Hepatitis C infection due to their relevance in the management of these cases with interferon therapy.

Published

1996

39. Investigation for VP4 Resion of Coxsackie Virus A16 RNA Sequence from Hand-Foot-Mouth Disease Patients at Eastern District of Shizuoka Prefecture in 1995

Author

Yutaka Arimoto, Koukichi Kawada, Tadaomi Tokutake, Kouzou Kanki, Keishi Hata, Goshima T, Tatsuo Kato, Yutaka Minohara, Akiko Kitamura, Hiroaki Ishiko, Naokazu Takeda, Yasushi Uchida, Fumie Goshima, Akio Hayashi, Natsuki Nakajima, and Hirofumi Kaku

Subjects

Male, Base Sequence, Molecular Sequence Data, Pcr cloning, Hand foot mouth disease, Infant, RNA, General Medicine, Biology, Polymerase Chain Reaction, Virology, Pediatric clinic, Virus, Reverse transcription polymerase chain reaction, Viral Proteins, Terminator (genetics), RNA Sequence, Humans, RNA, Viral, Female, Amino Acid Sequence, Child, Hand, Foot and Mouth Disease, Enterovirus

Abstract

In 1995 an investigation was made for VP4 regions of coxsackie virus A16 (CA16) RNA sequence from hand-foot-mouth disease patients in eastern district of Shizuoka Prefecture. Subjects were seven patients who were diagnosed as hand-foot-mouth disease due to CA16 at the Ohashi Pediatric Clinic in Susono City. Throat swabs of patients were extracted to RNA. Extracted RNA were assayed by reverse transcription polymerase chain reaction that primers corresponded to VP4 resion of enteroviruses. PCR products were marked by dye-deoxy terminator methods and assayed by direct sequence methods. RNA sequences were classified into two types. Type 1 were three cases, and type 2 were four. The homology was 90.8% between type 1 and type 2. All cases of sixty-nine amino acids were the same as prototype strain. We concluded that the two type strains of CA16 were prevalented in eastern district of Shizuoka Prefecture in 1995. It was at the same time and was widely noted in the eastern district.

Published

1996

40. Relation between serum hepatitis C virus-RNA levels and efficacy of interferon-β therapy

Author

Kouzou Kanki, Natsuki Nakajima, Yutaka Minohara, Yutaka Arimoto, Fumie Goshima, Hiroaki Ishiko, Toshiro Goshima, Tatsuo Kato, and Hilohumi Kaku

Subjects

Adolescent, business.industry, Hepatitis C virus, Hepacivirus, Interferon-beta, Hepatitis C, medicine.disease_cause, medicine.disease, Antiviral Agents, Chronic hepatitis, Interferon β, Interferon, Hepatitis C virus RNA, Chronic Disease, Pediatrics, Perinatology and Child Health, Immunology, medicine, Humans, RNA, Viral, Female, Alanine aminotransferase, business, Complete response, medicine.drug

Abstract

We performed two courses of interferon-beta (IFN-beta) to a child with chronic hepatitis C. A complete response was not obtained by the first interferon treatment, however, the results of the second treatment differed from those of the first. Hepatitis C virus (HCV)-RNA remained negative and both aspartate aminotransferase and alanine aminotransferase levels remained normal after completion of the second course. From these results we estimated that HCV-RNA levels before IFN therapy could be significantly associated with the efficacy of this treatment. The serum level of HCV-RNA was 10(6) copies/50 microL before the first treatment, but was 10(3) copies/50 microL before the second course. We conclude that IFN therapy to children with hepatitis C should always be directed at providing a cure. Even if the clinical effects of the first course are minimal decreasing quantities of HCV-RNA still offer hope for cure by subsequent readministration.

Published

1995

41. Familial Clustering Case of Hepatitis Delta

Author

Yutaka MINOHARA, Tatsuo KATO, Kouzou KANKI, Toshirou GOSHIMA, Natsuki NAKAJIMA, Hirofumi KAKU, Yutaka ARIMOTO, Fumie GOSHIMA, Keiji DOI, Kouichi SAITOH, Yoshihiko OOTSUKA, and Hiroaki ISHIKO

Subjects

Family Health, Male, HEPATITIS DELTA, Familial clustering, General Medicine, Hepatitis B, Biology, medicine.disease, Virology, Hepatitis D, law.invention, Serology, Antigen, law, Specific primers, medicine, Cluster Analysis, Humans, Female, Child, Polymerase chain reaction

Abstract

We report a familial clustering case of hepatitis delta. All of the members of this family had evidence of past infection of hepatitis B. We investigated the hepatitis delta, three of the members had positive serological hepatitis delta markers. We assayed by polymerase chain reaction the primers corresponding to hepatitis delta antigen. The results of polymerase chain reaction was three positive. The 2nd polymerase chain reaction was used, two geno-type specific primers one was for Japanese S type the other was for Japanese M type7). Three were positive the 2nd polymerase chain reaction for Japanese M, one was negative for all of hepatitis delta polymerase chain reaction.

Published

1995

42. A retrospective study on imported hepatitis E in Japan

Author

Hiroaki Ishiko, Naokazu Takeda, Tatsuo Miyamura, Tian-Cheng Li, Susumu Ochiai, and Takaji Wakita

Subjects

Adult, Male, medicine.medical_specialty, Adolescent, Genotype, viruses, Enzyme-Linked Immunosorbent Assay, medicine.disease_cause, Antibodies, Viral, Young Adult, Hepatitis E virus, Japan, Disease Transmission, Infectious, Medicine, Travel medicine, Humans, Aged, Retrospective Studies, Hepatitis, Travel, Acute hepatitis E, business.industry, Reverse Transcriptase Polymerase Chain Reaction, Public Health, Environmental and Occupational Health, virus diseases, Retrospective cohort study, Middle Aged, medicine.disease, Hepatitis E, Virology, digestive system diseases, Infectious Diseases, Immunoglobulin M, RNA, Viral, Female, Human hepatitis, business, Acute hepatitis

Abstract

Summary Hepatitis E virus (HEV), a causative agent of human hepatitis E, is transmitted through an oral-fecal route, often by contaminated drinking water. Serum specimens were collected from 112 non-A, -B, and –C acute hepatitis patients from 1989 to 2004 in Japan. Of these, 24 patients were found to be positive for anti-HEV IgM and diagnosed with acute Hepatitis E. Seventeen of these patients had a clear history of traveling abroad before disease onset and were counted as cases of imported HEV infection. HEV RNA was detected in 16 of these imported cases, and the nucleotide sequences similar to those of HEV detected in India, Bangladesh, and China were identified. By phylogenetic analysis, the remaining imported case appeared to have been imported from India, even though the patient's travel history was uncertain. These results indicated that some sporadic cases of hepatitis E in Japan are caused by imported HEV, and that phylogenetic analyses enable us to identify the country or area where a patient has been infected.

Published

2011

43. Selection of Mycoplasma genitalium strains harbouring macrolide resistance-associated 23S rRNA mutations by treatment with a single 1 g dose of azithromycin

Author

Takashi Deguchi, Yasushi Shimada, Shinichi Ito, Shigeaki Yokoi, Mitsuru Yasuda, Shin Ito, Yuko Yamaguchi, Masahiro Nakano, and Hiroaki Ishiko

Subjects

Male, Genotype, Single-nucleotide polymorphism, Mycoplasma genitalium, Dermatology, Microbial Sensitivity Tests, Azithromycin, urologic and male genital diseases, medicine.disease_cause, Polymorphism, Single Nucleotide, Microbiology, 23S ribosomal RNA, Drug Resistance, Bacterial, medicine, Humans, Urethritis, Mycoplasma Infections, Escherichia coli, Genotyping, Gene, biology, bacterial infections and mycoses, biology.organism_classification, medicine.disease, Virology, female genital diseases and pregnancy complications, Anti-Bacterial Agents, RNA, Bacterial, Infectious Diseases, RNA, Ribosomal, Mutation, Macrolides, medicine.drug

Abstract

Objective A single 1 g dose regimen of azithromycin has been recommended for the treatment of Mycoplasma genitalium infections. The authors evaluated whether this regimen could select M genitalium strains with macrolide resistance after treatment for M genitalium -positive non-gonococcal urethritis. Methods In seven men with non-gonococcal urethritis, who were infected with M genitalium without macrolide resistance-associated mutations but experienced microbiological azithromycin treatment failure, M genitalium DNAs in their post-treatment urine specimens were examined for mutations in the 23S rRNA gene and the ribosomal protein genes of L4 and L22. To assess the relatedness of M genitalium strains before and after treatment, their DNAs in pretreatment and post-treatment urine were genotyped by analysing short tandem repeats of an AGT/AAT unit in the MG309 gene and single nucleotide polymorphisms in the MG191 gene. Results In four of seven patients, M genitalium in post-treatment urine had an A-to-G transition at nucleotide position 2071 or 2072, corresponding to 2058 or 2059 in the 23S rRNA gene of Escherichia coli . In one of the four strains, Pro81Ser in the ribosomal protein L4 accompanied the mutation in the 23S rRNA gene. The genotyping of M genitalium DNAs suggested that these four post-treatment strains were selected from the respective closely related or identical pretreatment strains without macrolide resistance-associated mutations by the treatment. Conclusions The single 1 g dose treatment of azithromycin could select M genitalium strains harbouring macrolide resistance-associated mutations. For M genitalium , this regimen might increase the risk of macrolide resistance selection after treatment.

Published

2011

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

Author

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

Subjects

Microbiology (medical), Adenoviridae Infections, Molecular Sequence Data, Keratoconjunctivitis, Sequence Homology, Genome, Viral, Biology, Genome, Virus, law.invention, Viral Proteins, Japan, law, Virology, Cluster Analysis, Humans, Gene, Phylogeny, Genetics, Whole genome sequencing, Molecular Epidemiology, Phylogenetic tree, Molecular epidemiology, Viral culture, Adenoviruses, Human, virus diseases, Sequence Analysis, DNA, eye diseases, DNA, Viral, Recombinant DNA

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.

Published

2011

45. Analysis of the gyrA and parC genes ofMycoplasma genitaliumdetected in first-pass urine of men with non-gonococcal urethritis before and after fluoroquinolone treatment

Author

Shigeaki Yokoi, Takashi Yoshida, Shin-ichi Maeda, Y Takahashi, Hiroaki Ishiko, Masayoshi Tamaki, Takashi Deguchi, Masayasu Ito, and Satoshi Ishihara

Subjects

DNA Topoisomerase IV, Male, Pharmacology, Microbiology (medical), First pass, biology, Urethritis, Non-gonococcal urethritis, Urine, biology.organism_classification, medicine.disease, Virology, Mycoplasma, Infectious Diseases, Anti-Infective Agents, DNA Gyrase, medicine, Humans, Mycoplasma Infections, Pharmacology (medical), Mycoplasma genitalium, Gene, Fluoroquinolones

Published

2001

46. A comparison of the VP1, VP2, and VP4 regions for molecular typing of human enteroviruses

Author

David, Perera, Hiroyuki, Shimizu, Hiromu, Yoshida, Phan Van, Tu, Hiroaki, Ishiko, Peter C, McMinn, and Mary J, Cardosa

Subjects

Viral Structural Proteins, Polymorphism, Genetic, Genotype, Reverse Transcriptase Polymerase Chain Reaction, Humans, DNA Primers, Enterovirus

Abstract

The VP4, VP2, and VP1 gene regions were evaluated for their usefulness in typing human enteroviruses. Three published RT-PCR primers sets targeting separately these three gene regions were used. Initially, from a total of 86 field isolates (36 HEV-A, 40 HEV-B, and 10 HEV-C) tested, 100% concordance in HEV-A was identified from all three gene regions (VP4, VP2, and VP1). However, for HEV-B and HEV-C viruses, only the VP2 and VP1 regions, and not VP4, showed 100% concordance in typing these viruses. To evaluate further the usefulness of VP4 in typing HEV-A enteroviruses, 55 Japanese and 203 published paired VP4 and VP1 nucleotide sequences were also examined. In each case, typing by VP4 was 100% in concordance with typing using VP1. Given these results, it is proposed that for HEV-A enteroviruses, all three gene regions (VP4, VP2, and VP1), would be useful for typing these viruses. These options would enhance the capability of laboratories in identifying these viruses and would greatly help in outbreaks of hand, foot, and mouth disease.

Published

2010

47. Phylogenetic analysis of a coxsackievirus A24 variant: The most recent worldwide pandemic was caused by progenies of a virus prevalent around 1981

Author

Nobuko Kato, Masako Tanimura, John S. Tam, Shudo Yamazaki, Hiroaki Ishiko, Yin-Murphy M, Naokazu Takeda, Kikuko Miyamura, Gui-Fan Mu, and Kuei-Hsiang Lin

Subjects

Molecular Sequence Data, Coxsackievirus Infections, Biology, medicine.disease_cause, Polymerase Chain Reaction, Virus, Disease Outbreaks, Phylogenetics, Virology, medicine, Amino Acid Sequence, Cloning, Molecular, Phylogeny, Enterovirus, Genetics, Base Sequence, Phylogenetic tree, Molecular epidemiology, UPGMA, Nucleic acid sequence, Acute hemorrhagic conjunctivitis, medicine.disease, Oligodeoxyribonucleotides, Conjunctivitis, Acute Hemorrhagic, Sequence Alignment

Abstract

Nucleotide substitutions in the viral-encoded proteinase 3C (3Cpro) region (549 nucleotides) of the RNA genome of a coxsackievirus A24 variant (CA24v), one of the agents causing acute hemorrhagic conjunctivitis (AHC), were studied using 32 isolates collected from the Eastern hemisphere in 1970-1989. Based on regression analysis of nucleotide differences among isolates, the nucleotide substitution rate of CA24v 3Cpro was estimated to be 3.7 x 10(-3)/nucleotide/year. A phylogenetic tree constructed by the modified unweighted pair group method using arithmetic averages (UPGMA) indicated that CA24v had evolved from a common ancestor which appeared in one focal place in November 1963 +/- 21 months, about 7 years before the first isolation of CA24v in Singapore. The tree also revealed that all the recent epidemic isolates in 1985-1989 including Asian and Ghanian strains diverged from each other after 1981. This finding is consistent with the evidence that AHC due to CA24v had been confined to Southeast Asia and the Indian subcontinent until 1985, then suddenly and explosively spread to other areas where no CA24v isolations had been reported.

Published

1992

48. Molecular Cloning, Expression, and Antigenicity of Seto Virus Belonging to Genogroup I Norwalk-Like Viruses

Author

Shinichi Kobayashi, Kenji Sakae, Kuniko Shinozaki, Katsuro Natori, Kenji Suzuki, Kunio Kamata, Tatsuo Miyamura, Mineyuki Okada, Yasumoto Suzuki, Hiroaki Ishiko, and Naokazu Takeda

Subjects

Microbiology (medical), Antigenicity, viruses, Molecular Sequence Data, Heterologous, Enzyme-Linked Immunosorbent Assay, Molecular cloning, Virus, law.invention, Microbiology, Feces, Capsid, fluids and secretions, law, Virology, Animals, Humans, Cloning, Molecular, Antigens, Viral, Caliciviridae Infections, biology, Reverse Transcriptase Polymerase Chain Reaction, virus diseases, respiratory system, biology.organism_classification, Recombinant Proteins, Caliciviridae, Gastroenteritis, Blotting, Southern, Norwalk virus, Recombinant DNA, Rabbits

Abstract

The viral capsid protein of the Seto virus (SeV), a Japanese strain of genogroup I Norwalk-like viruses (NLVs), was expressed as virus-like particles using a baculovirus expression system. An antigen detection enzyme-linked immunosorbent assay based on hyperimmune antisera to recombinant SeV was highly specific to homologous SeV-like strains but not heterologous strains in stools, allowing us type-specific detection of NLVs.

Published

2000

49. Spread of epidemic keratoconjunctivitis due to a novel serotype of human adenovirus in Japan

Author

Koki Aoki and Hiroaki Ishiko

Subjects

Microbiology (medical), Serotype, viruses, Adenoviridae Infections, Molecular Sequence Data, Keratoconjunctivitis, Sequence Homology, medicine.disease_cause, Virus, Microbiology, Japan, medicine, Humans, Letters to the Editor, Phylogeny, biology, Adenoviruses, Human, virus diseases, Sequence Analysis, DNA, medicine.disease, biology.organism_classification, Virology, eye diseases, Epidemic Keratoconjunctivitis, Adenoviridae, Mastadenovirus, DNA, Viral, Viral disease

Abstract

We have reported a novel human adenovirus (HAdV) that has caused a nationwide epidemic of keratoconjunctivitis (EKC) in Japan ([11][1]). This virus has been characterized serologically and genetically as a novel serotype, and we propose naming it HAdV-54. The GenBank accession number of the

Published

2009

50. [Guideline for the nosocomial infections of adenovirus conjunctivitis]

Author

Hiroshi, Shiota, Shigeaki, Ohno, Koki, Aoki, Atsushi, Azumi, Hiroaki, Ishiko, Yoshitsugu, Inoue, Norio, Usui, Eiichi, Uchio, Hisatoshi, Kaneko, Shigeto, Kumakura, Yoshitsugu, Tagawa, Yasuhiro, Tanifuji, Hisashi, Nakagawa, Rikutaro, Hinokuma, Shudo, Yamazaki, and Norihiko, Yokoi

Subjects

Adenovirus Infections, Human, Disinfection, Conjunctivitis, Viral, Cross Infection, Adrenal Cortex Hormones, Practice Guidelines as Topic, Humans, Ophthalmic Solutions, Serotyping, Antiviral Agents, Adenoviridae, Disinfectants

Published

2009