The antiviral enzymes PKR and RNase L suppress gene expression from viral and non-viral based vectors.
AUTOR(ES)
Terenzi, F
RESUMO
Expression of transfected genes is shown to be suppressed by two intracellular enzymes, RNase L and protein kinase PKR, which function in interferon-treated cells to restrict viral replication. RNase L(-/-) or PKR(-/-) murine embryonic fibroblasts produced enhanced levels of protein from transfected genes compared with wild-type cells. Increased expression of exogenous genes in RNase L(-/-) cells correlated with elevated levels of mRNA and thus appeared to be due to enhanced mRNA stability. Plasmid encoding adenovirus VA RNAs was able to further enhance accumulation of the exogenous gene transcript and protein, even in cells lacking PKR. In contrast to the increased expression of transfected genes in cells lacking RNase L or PKR, expression of endogenous host genes was unaffected by the absence of these enzymes. In addition, a dominant-negative PKR mutant improved expression from a conventional plasmid vector and from a Semliki Forest virus derived, self-replicating vector. These results indicate that viral infections and transfections produce similar stress responses in mammalian cells and suggest strategies for selectively increasing expression of exogenous genes.
ACESSO AO ARTIGO
http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=148718Documentos Relacionados
- Cholesterol improves the transfection efficiency of polyallylamine as a non-viral gene delivery vector
- Close relationship between non-viral retroposons in Drosophila melanogaster.
- Preparation and characterization of non-viral gene delivery systems with pEGFP-C1 Plasmid DNA
- Novel non-viral method for transfection of primary leukemia cells and cell lines
- Gene expression from transcriptionally disabled retroviral vectors.
