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Inhibition of hepatitis B virus DNA replication by a thermostable interferon-γ variant
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Background Treatment of HBV chronic carriers using interferon (IFN)-α or nucleoside/nucleotide analogues fails to suppress viral infection. Type-II IFN-γ has been shown to inhibit HBV replication. The goal of the present work was to evaluate the antiviral efficacy against HBV of a thermostable IFN-γ variant isolated using Massive Mutagenesis® and thermoresistant selection (THR™) technologies. Methods The thermostability of wild-type (wt) and S63C IFN-γ was determined in vitro and in vivo. Activation of the IFN-γ responsive element by wt and S63C IFN-γ was tested using a luciferase assay. HepG2.2.15 cells constitutively expressing HBV were used to analyse the antiviral activity of wt and S63C IFN-γ against HBV replication. Intracellular HBV DNA was detected by Southern blot and quantified by real-time PCR analyses. Results S63C IFN-γ was shown to be more thermostable and had a longer half-life than wt IFN-γ. Both wt and S63C IFN-γ displayed a similar capacity to activate the IFN pathway. The treatment of HepG2.2.15 cells with wt or S63C IFN-γ induced the inhibition of HBV viral replication. After heating, S63C IFN-γ displayed better conservation of its antiviral activity against HBV when compared with wt IFN-γ. Conclusions These results confirm that the THR™ method can be used to isolate mutants with enhanced thermostability and demonstrate that a thermostable IFN-γ variant presents antiviral properties against HBV replication. This molecule could provide a new strategy to treat patients who do not respond to antiviral therapy.
Title: Inhibition of hepatitis B virus DNA replication by a thermostable interferon-γ variant
Description:
Background Treatment of HBV chronic carriers using interferon (IFN)-α or nucleoside/nucleotide analogues fails to suppress viral infection.
Type-II IFN-γ has been shown to inhibit HBV replication.
The goal of the present work was to evaluate the antiviral efficacy against HBV of a thermostable IFN-γ variant isolated using Massive Mutagenesis® and thermoresistant selection (THR™) technologies.
Methods The thermostability of wild-type (wt) and S63C IFN-γ was determined in vitro and in vivo.
Activation of the IFN-γ responsive element by wt and S63C IFN-γ was tested using a luciferase assay.
HepG2.
2.
15 cells constitutively expressing HBV were used to analyse the antiviral activity of wt and S63C IFN-γ against HBV replication.
Intracellular HBV DNA was detected by Southern blot and quantified by real-time PCR analyses.
Results S63C IFN-γ was shown to be more thermostable and had a longer half-life than wt IFN-γ.
Both wt and S63C IFN-γ displayed a similar capacity to activate the IFN pathway.
The treatment of HepG2.
2.
15 cells with wt or S63C IFN-γ induced the inhibition of HBV viral replication.
After heating, S63C IFN-γ displayed better conservation of its antiviral activity against HBV when compared with wt IFN-γ.
Conclusions These results confirm that the THR™ method can be used to isolate mutants with enhanced thermostability and demonstrate that a thermostable IFN-γ variant presents antiviral properties against HBV replication.
This molecule could provide a new strategy to treat patients who do not respond to antiviral therapy.
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