Publication | Open Access
Attenuated protein expression vectors for use in siRNA rescue experiments
53
Citations
15
References
2012
Year
Viral ReplicationImmunologyMolecular BiologyTransient TransfectionSirna Target SpecificitySirna TransfectionProtein ExpressionHuman RetrovirusSirna Rescue ExperimentsVirologyHivGene ExpressionFunctional GenomicsCell BiologyBioinformaticsNatural SciencesAntiviral ResponseProtein EngineeringGene VectorSmall RnaSystems BiologyMedicineGenome Editing
Transient transfection of small interfering RNA (siRNA) provides a powerful approach for studying cellular protein functions, particularly when the target protein can be re-expressed from an exogenous siRNA-resistant construct in order to rescue the knockdown phenotype, confirm siRNA target specificity, and support mutational analyses. Rescue experiments often fail, however, when siRNA-resistant constructs are expressed at suboptimal levels. Here, we describe an ensemble of mammalian protein expression vectors with CMV promoters of differing strengths. Using CHMP2A rescue of HIV-1 budding, we show that these vectors can combine high-transfection efficiencies with tunable protein expression levels to optimize the rescue of cellular phenotypes induced by siRNA transfection.
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