Abstract:pCB302-3 is a plant mini-binary stable transformation vector.To investigate the transient expression of pCB302-3 vector in plant,GFP was inserted into pCB302-3 vector as a reporter gene,and various factors including density of Agrobacterium cell,supplementation of gene silencing suppression p19 and days post infiltration were optimized based on agroinfiltration method in Nicotiana benthamiana leaves.Results showed that high levels of GFP expression were observed in N.benthamiana leaves 3-5 d after infiltration by Agrobacterium cell suspension contained pCB302-3-GFP with an optical density (D600) of 0.8-1.0 co-infiltrated with p19 gene.