Recombinant allergenic proteins have been produced in a variety of different expression systems. Plants and plant cells are now considered as viable and competitive expression systems for large-scale protein production. In this research, the plantlet of transgenic tobacco contained CaMV 35S promoter chimeric with Dermatophagoides pteronyssinus 2 (Der p 2) gene was used to induce formation of callus and hairy roots, and cultures of suspension cell and hairy root were studied for recombinant Der p 2 production. By Der p 2 sandwich enzyme-linked immunosorbent assay (sandwich-ELISA), cell line-D3 expressed the highest Der p 2 productivity in 8 suspension cell lines. The cultivation of S3 in flasks showed the maximum productivity, 788.3 μg/ L, at 16th d; batch culture of S3 in bioreactor reached the highest productivity, 515.1μg/L, at 8th d. Induction of hairy roots from transgenic tobacco, 24 cell lines was established. Maximum productivity, 475.2 ng/mL of Der p 2 was produced in flask within 30 d by R19. In this work, we constructed the chimeric gene of HSP 18.2 inducible promoter fused with Der p 2, and successfully expressed it in tobacco hairy roots by heat treatment. After the treatment of ammonia sulfate precipitation, cation exchange chromatography (SP Sephadex), and monoclonal anti-Der p 2 affinity column, recombinant Der p 2 protein was purified into homologous, the recovery rate was 19.7 %.