Analysis of in vitro replicated human hepatitis C virus (HCV) for the determination of genotypes and quasispecies

doi:10.1186/1743-422X-3-81

Virology Journal

Volume 3

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Revie D
Alberti MO
Braich RS
Chelyapov N
Bayles D
Prichard JG
Salahuddin SZ

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Alberti MO
Braich RS
Chelyapov N
Bayles D
Prichard JG
Salahuddin SZ
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Analysis of in vitro replicated human hepatitis C virus (HCV) for the determination of genotypes and quasispecies

Dennis Revie¹ , Michael O Alberti¹ , Ravi S Braich²^,4 , Nickolas Chelyapov²^,5 , David Bayles² , John G Prichard³ and S Zaki Salahuddin²

¹Department of Biology, California Lutheran University, Thousand Oaks, California, USA

²California Institute of Molecular Medicine, Ventura, California, USA

³Ventura County Medical Center, Ventura, California, USA

⁴Alnylam Pharmaceuticals, Cambridge, Massachusetts, USA

⁵University of Southern California, Los Angeles, California, USA

author email corresponding author email

Virology Journal 2006, 3:81doi:10.1186/1743-422X-3-81


Published:	29 September 2006

Abstract

Isolation and self-replication of infectious HCV has been a difficult task. However, this is needed for the purposes of developing rational drugs and for the analysis of the natural virus. Our recent report of an in vitro system for the isolation of human HCV from infected patients and their replication in tissue culture addresses this challenge. At California Institute of Molecular Medicine several isolates of HCV, called CIMM-HCV, were grown for over three years in cell culture. This is a report of the analysis of CIMM-HCV isolates for subtypes and quasispecies using a 269 bp segment of the 5'UTR. HCV RNA from three patients and eleven CIMM-HCV were analyzed for this purpose. All isolates were essentially identical. Isolates of HCV from one patient were serially transmitted into fresh cells up to eight times and the progeny viruses from each transmission were compared to each other and also to the primary isolates from the patient's serum. Some isolates were also transmitted to different cell types, while others were cultured continuously without retransmission for over three years. We noted minor sequence changes when HCV was cultured for extended periods of time. HCV in T-cells and non-committed lymphoid cells showed a few differences when compared to isolates obtained from immortalized B-cells. These viruses maintained close similarity despite repeated transmissions and passage of time. There were no subtypes or quasispecies noted in CIMM-HCV.