Expression efficiency of green fluorescent protein ( GFP ) in hairy root cultures of Nicotiana tabacum by different gene construction designs was compared. These gene constructions including gfp driven by CaMV 35S promoter ( pCAMBIA 1302 ), then further fused with signal sequence to the 5’ of gfp ( pCSP ), and then further fused with ER-retaintion sequence to the 3’ of gfp ( pCSP-KDEL ). Establishment of Nicotiana tabacum transgenic hairy roots was achieved by Agrobacterium rhizogenes-mediated transformation, PCR confirmation, fluorescence microscopy observation, Western blot of GFP and its ELISA assay. Clone of CY A3, SP F3 and KDEL J3 was selected from each design for GFP expression comparison. After 28-d cultivation, the expressed GFP of the three constructions was 985.5, 258.9 and 54.2 ng / 50 mL, respectively, and the ratio of GFP secreted was 21, 33, and 40%, respectively. Among the three constructions, our results reveal that gene construction without secretion designs possessed the highest GFP expression efficiency, although SP and KDEL designs showed higher ratio of GFP in the cultured medium. In the experiment of enzymatic lysis of transgenic hairy roots cell wall, the released GFP of three transgenic line CY A3, SP F3 and KDEL J3 was 20%, 27% and 35% of the total cytosol GFP , respectively. It suggests that secretion of GFP in the design of SP and KDEL might be hindered by cell wall layer.