Literature DB >> 8904426

Rapid subgenus identification of human adenovirus isolates by a general PCR.

A H Kidd1, M Jonsson, D Garwicz, A E Kajon, A G Wermenbol, M W Verweij, J C De Jong.   

Abstract

In most clinical situations involving adenovirus infection, subgenus (subgroup) identification of an adenovirus isolate is as informative as a finer identification by serotype. A PCR method which allows the identification of human adenovirus isolates as members of subgenera A, B:1, B:2, C, D, E, or F is described. It is based on a simple (nonnested) PCR using primers which bind to regions immediately flanking the VA RNA-encoding regions of human adenovirus genomes. The PCR allows amplification of DNA from all 49 human adenovirus prototype strains so far described. Since there are differences in the lengths of the VA RNA-encoding regions in adenoviruses of different subgenera, it is possible to differentiate some subgenera according to the size of the PCR product determined by electrophoresis. This forms the basis of an initial broad categorization of isolates as belonging to either (i) subgenus B:1, C, D, or E or (ii) subgenus A, B:2, or F. Subgenus identification is completed by a one-step restriction enzyme digestion and gel electrophoresis. The method was assessed by blind subgenus identification of 200 miscellaneous primate adenovirus isolates prepared by the reference laboratory at Bilthoven, The Netherlands. Identification at the subgenus level by PCR correlated 91.5% with the results of serotyping. A further 5.5% of isolates were correctly identified as belonging to one of two specified subgenera. Six of the 200 identifications (3%) were unsuccessful for various reasons, including weak PCR products, intermediate strains, and mistaken primate host. The method should serve as a rapid means of confirming adenovirus cytopathic effects in laboratories performing virus culture, with simultaneous subgenus identification of the isolate. It will also have relevance as an aid to conventional serotyping for epidemiological purposes, since for all adenoviruses except those belonging to subgenus D, neutralization tests need only involve a maximum of four type-specific antisera.

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Year:  1996        PMID: 8904426      PMCID: PMC228858          DOI: 10.1128/jcm.34.3.622-627.1996

Source DB:  PubMed          Journal:  J Clin Microbiol        ISSN: 0095-1137            Impact factor:   5.948


  35 in total

1.  Monoclonal antibody enzyme-linked immunosorbent assay for specific identification and typing of subgroup F adenoviruses.

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2.  Recombination in adenovirus: crossover sites in intertypic recombinants are located in regions of homology.

Authors:  M E Boursnell; V Mautner
Journal:  Virology       Date:  1981-07-15       Impact factor: 3.616

Review 3.  Genetic variability of adenoviruses.

Authors:  G Wadell; M L Hammarskjöld; G Winberg; T M Varsanyi; G Sundell
Journal:  Ann N Y Acad Sci       Date:  1980       Impact factor: 5.691

4.  Worldwide epidemiology of human adenovirus infections.

Authors:  H Schmitz; R Wigand; W Heinrich
Journal:  Am J Epidemiol       Date:  1983-04       Impact factor: 4.897

5.  Faecal adenoviruses from Glasgow babies. Studies on culture and identity.

Authors:  A H Kidd; B P Cosgrove; R A Brown; C R Madeley
Journal:  J Hyg (Lond)       Date:  1982-06

6.  Antigenic characterization of intermediate adenovirus 14-11 strains associated with upper respiratory illness in a military camp.

Authors:  J C Hierholzer; A Pumarola
Journal:  Infect Immun       Date:  1976-02       Impact factor: 3.441

7.  The Seattle Virus Watch. VII. Observations of adenovirus infections.

Authors:  J P Fox; C E Hall; M K Cooney
Journal:  Am J Epidemiol       Date:  1977-04       Impact factor: 4.897

8.  Direct identification of enteric adenovirus, a candidate new serotype, associated with infantile gastroenteritis.

Authors:  M E Johansson; I Uhnoo; A H Kidd; C R Madeley; G Wadell
Journal:  J Clin Microbiol       Date:  1980-07       Impact factor: 5.948

9.  Infections in 18,000 infants and children in a controlled study of respiratory tract disease. I. Adenovirus pathogenicity in relation to serologic type and illness syndrome.

Authors:  C D Brandt; H W Kim; A J Vargosko; B C Jeffries; J O Arrobio; B Rindge; R H Parrott; R M Chanock
Journal:  Am J Epidemiol       Date:  1969-12       Impact factor: 4.897

10.  Candidate adenoviruses 40 and 41: fastidious adenoviruses from human infant stool.

Authors:  J C de Jong; R Wigand; A H Kidd; G Wadell; J G Kapsenberg; C J Muzerie; A G Wermenbol; R G Firtzlaff
Journal:  J Med Virol       Date:  1983       Impact factor: 2.327

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  26 in total

1.  Rapid typing of human adenoviruses by a general PCR combined with restriction endonuclease analysis.

Authors:  A Allard; B Albinsson; G Wadell
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2.  Relevance of commercial diagnostic tests to detection of enteric adenovirus infections in South Africa.

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3.  PCR and restriction endonuclease analysis for rapid identification of human adenovirus subgenera.

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4.  Phylogenetic analysis of the main neutralization and hemagglutination determinants of all human adenovirus prototypes as a basis for molecular classification and taxonomy.

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Review 6.  Molecular typing of enteroviruses: current status and future requirements. The European Union Concerted Action on Virus Meningitis and Encephalitis.

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7.  Two adenovirus serotype 3 outbreaks associated with febrile respiratory disease and pharyngoconjunctival fever in children under 15 years of age in Hangzhou, China, during 2011.

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8.  Molecular detection and quantitative analysis of the entire spectrum of human adenoviruses by a two-reaction real-time PCR assay.

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9.  PCR detection of adenovirus in a bone marrow transplant recipient: hemorrhagic cystitis as a presenting manifestation of disseminated disease.

Authors:  M S Echavarria; S C Ray; R Ambinder; J S Dumler; P Charache
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10.  Use of oligonucleotide microarrays for rapid detection and serotyping of acute respiratory disease-associated adenoviruses.

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Journal:  J Clin Microbiol       Date:  2004-07       Impact factor: 5.948

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