Literature DB >> 14522064

A comparison of methods for detecting adenovirus type 8 keratoconjunctivitis during a nosocomial outbreak in a Neonatal Intensive Care Unit.

Elena Percivalle1, Antonella Sarasini, Maria Torsellini, Loredana Bruschi, Elena Antoniazzi, M Grazia Revello, Giuseppe Gerna.   

Abstract

BACKGROUND: An outbreak of epidemic keratoconjunctivitis (EKC) due to adenovirus (Ad) type 8 and involving 14 members of the hospital staff and 33 neonates admitted to the Neonatal Intensive Care Unit of the local University Hospital occurred between September and December 2000 in Pavia, Italy. The outbreak was preceded by an outbreak of EKC within the community.
OBJECTIVE: To compare the performance of conventional virus isolation on cell cultures, direct detection of Ad antigens in conjunctival cells by a direct fluorescent assay (DFA) and Ad DNA detection in conjunctival swabs by polymerase chain reaction (PCR) for diagnosis of adenoviral conjunctivitis. STUDY
DESIGN: Of conjunctival swabs collected from 47 patients, all were tested by virus isolation, 43 by direct Ad antigen detection, and 37 by Ad DNA detection. Direct Ad antigen detection was carried out by DFA using a group-specific monoclonal antibody. Detection and subgrouping of Ad DNA by nested PCR was performed using two sets of primers complementary to hexon and fiber genes, respectively.
RESULTS: Ad was detected in 24/47 (51.1%), 21/43 (48.8%), and 23/37 (62.1%) samples by virus isolation, direct antigen detection and PCR, respectively. Overall, 30/47 (63.8%) samples were Ad-positive. Of 37 specimens tested in parallel by all three methods, Ad was detected by at least one of the three techniques in 26/37 (70.3%). All Ad isolates were identified as serotype 8 by neutralization, while all PCR-positive samples were identified as belonging to subgroup D. No other virus was isolated from any conjunctival swab. Time required for test completion was 9.6 (4-20) days for virus isolation, 1-2 h for DFA and 24 h for PCR.
CONCLUSIONS: DFA was a sensitive and rapid assay but results depend on the quality of sample and the expertise of the observer. PCR was the most sensitive assay, although it takes longer to perform and requires dedicated facilities; thus, it could be restricted to DFA-negative samples. Virus isolation is still useful from an epidemiological point of view.

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Year:  2003        PMID: 14522064     DOI: 10.1016/s1386-6532(03)00011-8

Source DB:  PubMed          Journal:  J Clin Virol        ISSN: 1386-6532            Impact factor:   3.168


  8 in total

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2.  Role of molecular diagnostics in ocular microbiology.

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Journal:  Curr Ophthalmol Rep       Date:  2013-12-01

3.  Conjunctivitis: systematic approach to diagnosis and therapy.

Authors:  Onsiri Thanathanee; Terrence P O'Brien
Journal:  Curr Infect Dis Rep       Date:  2011-04       Impact factor: 3.725

4.  Rapid detection of oculopathogenic adenovirus in conjunctivitis.

Authors:  Maysaa El-Sayed Zaki; Ghada A Abd-El Fatah
Journal:  Curr Microbiol       Date:  2007-11-06       Impact factor: 2.188

5.  Molecular epidemiology of adenoviral keratoconjunctivitis in Saudi Arabia.

Authors:  Khalid F Tabbara; Nazri Omar; Ehab Hammouda; Masataka Akanuma; Takeshi Ohguchi; Toshihide Ariga; Yoshitsugu Tagawa; Nobuyoshi Kitaichi; Susumu Ishida; Koki Aoki; Hiroaki Ishiko; Shigeaki Ohno
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6.  Outbreak of epidemic keratoconjunctivitis caused by human adenovirus type 56, China, 2012.

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Review 7.  Adenovirus: Epidemiology, Global Spread of Novel Serotypes, and Advances in Treatment and Prevention.

Authors:  Joseph P Lynch; Adriana E Kajon
Journal:  Semin Respir Crit Care Med       Date:  2016-08-03       Impact factor: 3.119

Review 8.  Recent Advances in Early Diagnosis of Viruses Associated with Gastroenteritis by Biosensors.

Authors:  Abouzar Babaei; Nastaran Rafiee; Behnaz Taheri; Hessamaddin Sohrabi; Ahad Mokhtarzadeh
Journal:  Biosensors (Basel)       Date:  2022-07-08
  8 in total

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