Two regions of an avian hepadnavirus RNA pregenome are required in cis for encapsidation

Author:

Calvert J1,Summers J1

Affiliation:

1. Department of Cell Biology, University of New Mexico School of Medicine Cancer, Research and Treatment Center, Albuquerque 87131.

Abstract

We have constructed a series of deletion mutants spanning the genome of duck hepatitis B virus in order to determine which regions of the viral genome are required in cis for packaging of the pregenome into capsid particles. Deletion of sequences within either of two nonadjacent regions prevented replication of the mutant viral genomes expressed in a permissive avian hepatoma cell line in the presence of functionally active viral core and P proteins. Extraction of RNA from cells transfected with these replication-defective mutants showed that the mutants retained the capacity to be transcribed into a pregenomic-size viral RNA, but that these RNA species were not packaged into viral capsids. The two regions defined by these deletions are located 36 to 126 (region I) and 1046 to 1214 (region II) nucleotides downstream of the 5' end of the pregenome and contain sequences which are required in cis for encapsidation of the duck hepatitis B virus pregenome.

Publisher

American Society for Microbiology

Subject

Virology,Insect Science,Immunology,Microbiology

Reference24 articles.

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2. The P gene product of hepatitis B virus is required as a structural component for genomic RNA encapsidation;Bartenschlager R.;J. Virol.,1990

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4. Hepatitis B virus nucleocapsid assembly: primary structure requirements in the core protein;Birnbaum F.;J. Virol.,1990

5. Naturally occurring point mutation in the C terminus of the polymerase gene prevents duck hepatitis B virus RNA packaging;Chen Y.;J. Virol.,1992

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