Quantitative Detection of Hepadnavirus-Infected Lymphoid Cells by In Situ PCR Combined with Flow Cytometry: Implications for the Study of Occult Virus Persistence

doi:10.1128/JVI.77.2.970-979.2003

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Journal of Virology, January 2003, p. 970-979, Vol. 77, No. 2
0022-538X/03/$08.00+0 DOI: 10.1128/JVI.77.2.970-979.2003
Copyright © 2003, American Society for Microbiology. All Rights Reserved.

Quantitative Detection of Hepadnavirus-Infected Lymphoid Cells by In Situ PCR Combined with Flow Cytometry: Implications for the Study of Occult Virus Persistence

Patricia M. Mulrooney¹ and Tomasz I. Michalak¹^,2^*

Molecular Virology and Hepatology Research, Division of Basic Medical Sciences,¹ Division of Pathology, Faculty of Medicine, Memorial University of Newfoundland, St. John's, Newfoundland, Canada A1B 3V6²

Received 21 August 2002/ Accepted 16 October 2002

The detection of small amounts of viral pathogens in infectedcells by classical PCR is hampered by a partial loss of virusnucleic acid due to extraction and by difficulties in discriminationbetween truly intracellular virus genome material and that possiblyadhered to the cell surface. These impediments limit reliableidentification of virus traces within infected cells, whichare typically encountered in latent and persistent occult infections.In this study, hepadnavirus-specific in situ PCR combined withthe enzymatic elimination of extracellular virus and flow cytometrypermitted detection of viral genomes in lymphoid cells withoutnucleic acid isolation and allowed quantification of infectedcells during the course of persistent infection with woodchuckhepatitis virus (WHV). The validity of the procedure was confirmedby hybridization analysis of the in situ-amplified viral sequences.The results showed that hepadnavirus can be directly detectedwithin lymphoid cells not only in serologically accountableinfection, but also years after recovery from viral hepatitisand in the course of primary occult virus carriage. Percentagesof infected peripheral lymphoid cells in symptomatic WHV hepatitisfluctuate between 3.4 and 20.4% (mean ± standard errorof the mean, 9.6% ± 1.7%), whereas those in persistent,serologically mute WHV infection range from 1.1 to 14.6% (mean± standard error of the mean, 4.8% ± 0.8%) (P= 0.005). The data obtained provide further evidence that WHVinfection continues indefinitely in the lymphatic system independentlyof whether it is symptomatic or concealed. They document thathepadnavirus can be detected in a significant proportion ofcirculating lymphoid cells in both immunovirologically apparentas well as occult persistent infection.

* Corresponding author. Mailing address: Molecular Virology and Hepatology Research, Division of Basic Medical Sciences, Faculty of Medicine, The Health Sciences Centre, Memorial University of Newfoundland, St. John's, NFLD, Canada A1B 3V6. Phone: (709) 777- 7301. Fax: (709) 777-8279. E-mail: timich{at}mun.ca.