Multiplex polymerase chain reaction for subgenus-specific detection of human adenoviruses in clinical samples

• Published in: Journal of medical virology Vol. 58; no. 1; pp. 87 - 92
• Main Authors: Pring-Åkerblom, Patricia, John Trijssenaar, F.E., Adrian, T., Hoyer, Hans
• Format: Journal Article
• Language: English
• Published: New York John Wiley & Sons, Inc 01.05.1999; Wiley-Liss
• Subjects: Adenovirus; Adenovirus Infections, Human - pathology; Adenovirus Infections, Human - virology; Adenoviruses, Human - genetics; Adenoviruses, Human - isolation & purification; Base Sequence; Biological and medical sciences; Capsid - genetics; Capsid Proteins; clinical applications; DNA Primers; DNA, Viral; epidemic keratoconjunctivitis; Fundamental and applied biological sciences. Psychology; gastroenteritis; Human adenovirus; Human viral diseases; Humans; Infectious diseases; Medical sciences; Microbiology; Molecular Sequence Data; Polymerase Chain Reaction - methods; Sensitivity and Specificity; Sequence Analysis, DNA; subgenus-specific primers; Techniques used in virology; Viral diseases; Viral diseases of the digestive system; Virology; Performance evaluation; Human; Adenoviridae; Multiple; Gastroenteritis; Infection; Virus; Polymerase chain reaction; Serotype specificity; Human adenovirus; Viral disease; Digestive diseases; Intestinal disease; Mastadenovirus; Diagnosis; Gastric disease
• ISSN: 0146-6615; 1096-9071
• DOI: 10.1002/(SICI)1096-9071(199905)58:1<87::AID-JMV14>3.0.CO;2-R

The polymerase chain reaction (PCR) has been used previously for the detection and typing of adenoviruses directly in clinical samples. Since under clinical conditions subgenus‐specific identification is often sufficient, we extended the genus‐ and type‐specific PCR by a subgenus‐specific PCR. By sequencing several loop l4 gene regions of the hexon (major adenovirus coat protein) and comparing them to published sequences, subgenus‐specific sequences were identified in this region. By using primers targeted to this region and to a conserved hexon gene region, a multiplex, nonnested PCR for the detection and subgenus‐specific identification of adenoviruses could be established. The six subgenus‐specific amplimers are distinguishable by agarose gel electrophoresis, and subsequent restriction analysis is not necessary. The specificity of the subgenus‐specific primer pairs was tested on 23 adenovirus prototypes, representing all six subgenera, on 9 subgenus B and D intermediate strains, and on 16 subgenus C genome types. Furthermore, multiplex, subgenus‐specific PCR was performed directly with 100 clinical specimens, including stool samples, ocular swabs, and throat swabs. Adenoviruses of all subgenera could be detected. Especially for clinical application, the rapid, one‐step differentiation between subgenus D adenoviruses, causing the severe and highly contagious epidemic keratoconjunctivitis, and subgenus B and E adenoviruses, causing relative harmless ocular infections, is of great importance. The subgenus‐specific PCR could also facilitate the primary classification of unknown virus isolates. J. Med. Virol. 58:87–92, 1999. © 1999 Wiley‐Liss, Inc.