Fig. 2
RYMVMg1ΔP1ΔCP/CterPSA RNA accumulation in Nicotiana benthamiana leaves. Semi-quantitative RT-PCR was performed on RNA extracted from N. benthamiana leaves infiltrated with either empty vector or RYMVMg1ΔP1ΔCP/CterPSA construct together with the cocktail of RNA silencing suppressors. Reverse transcriptions were performed using a mixture of oligodT and CterPSA specific primers. PCR amplification was performed using CterPSA-specific primers. NbEF1-α expression was used as internal control. Three independent experiments were performed. The results presented here are representative of the three experiments