Abstract
The propagation of the hepatitis C virus (HCV) is a complex process that requires both host and viral proteins. To facilitate identification of host cell factors that are required for HCV replication, we screened a panel of small interference RNAs that preferentially target human protein kinases using an HCV replicon expressing the firefly luciferase gene as a genetic reporter. Small interference RNAs specific for three human kinases, Csk, Jak1, and Vrk1, were identified that reproducibly reduce viral RNA and viral protein levels in HCV replicon-bearing cells. Treatment of replicon cells with a small molecule inhibitor of Csk also resulted in a significant reduction in HCV RNA and proteins, further supporting a role for Csk in HCV replication. The effects of siRNAs targeting eight kinases known to be negatively regulated by Csk were then examined; knock down of one of these kinases, Fyn, resulted in up-regulation of the HCV replicon, suggesting that Csk mediates its effect on HCV replication through Fyn. This conclusion was further corroborated by demonstration that replicon cells treated with Csk inhibitor contained lower levels of the phosphorylated form of Fyn than control cells.
Highlights
Lular and viral proteases into at least 10 individual structural and nonstructural (NS) proteins
Construction and Validation of a Selectable Tri-cistronic Subgenomic hepatitis C virus (HCV) Replicon Expressing the Firefly Luciferase Reporter—Several HCV replicon variants have been described previously that allow measurement of cellular replicon RNA levels through the activity of a reporter enzyme and, at the same time, harbor an antibiotic resistance gene that enables the selection of transfected cells with stably replicating HCV replicon RNA [12,13,14]
In parallel with these reports, we developed another HCV replicon, pFK-I389neo/luc/NS3-3Ј/5.1, which harbors the firefly luciferase gene and the Geneticin resistance gene neor
Summary
Lular and viral proteases into at least 10 individual structural and nonstructural (NS) proteins. Construction and Validation of a Selectable Tri-cistronic Subgenomic HCV Replicon Expressing the Firefly Luciferase Reporter—Several HCV replicon variants have been described previously that allow measurement of cellular replicon RNA levels through the activity of a reporter enzyme and, at the same time, harbor an antibiotic resistance gene that enables the selection of transfected cells with stably replicating HCV replicon RNA [12,13,14].
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