Prototype foamy virus protease activity is essential for intraparticle reverse transcription initiation but not absolutely required for uncoating upon host cell entry
Research output: Contribution to journal › Research article › Contributed › peer-review
Contributors
Abstract
Foamy viruses (FVs) are unique among retroviruses in performing genome reverse transcription (RTr) late in replication, resulting in an infectious DNA genome, and also in their unusual Pol biosynthesis and encapsidation strategy. In addition, FVs display only very limited Gag and Pol processing by the viral protease (PR) during particle morphogenesis and disassembly, both thought to be crucial for viral infectivity. Here, we report the generation of functional prototype FV (PFV) particles from mature or partially processed viral capsid and enzymatic proteins with infectivity levels of up to 20% of the wild type. Analysis of protein and nucleic acid composition, as well as infectivity, of virions generated from different Gag and Pol combinations (including both expression-optimized and authentic PFV open reading frames [ORFs]) revealed that precursor processing of Gag, but not Pol, during particle assembly is essential for production of infectious virions. Surprisingly, when processed Gag (instead of Gag precursor) was provided together with PR-deficient Pol precursor during virus production, infectious, viral DNA-containing particles were obtained, even when different vector or proviral expression systems were used. Although virion infectivity was reduced to 0.5 to 2% relative to that of the respective parental constructs, this finding overturns the current dogma in the FV literature that viral PR activity is absolutely essential at some point during target cell entry. Furthermore, it demonstrates that viral PR-mediated Gag precursor processing during particle assembly initiates intraparticle RTr. Finally, it shows that reverse transcriptase (RT) and integrase are enzymatically active in the Pol precursor within the viral capsid, thus enabling productive host cell infection.
Details
Original language | English |
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Pages (from-to) | 3163-3176 |
Number of pages | 14 |
Journal | Journal of Virology |
Volume | 87 |
Issue number | 6 |
Publication status | Published - Mar 2013 |
Peer-reviewed | Yes |
External IDs
PubMedCentral | PMC3592149 |
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ORCID | /0000-0002-0320-4223/work/150885042 |
Scopus | 84875298481 |
Keywords
Keywords
- Aspartic Acid Endopeptidases/metabolism, Cell Line, Humans, Reverse Transcription, Spumavirus/enzymology, Virion/chemistry, Virus Uncoating