Podophyllotoxin possesses strong tumor-specific cytotoxicity, and its chemical derivatives have been employed in clinical cancer treatment. From Podophyllum pleianthum Hance, pinoresinol lariciresinol reductase (PLR) gene was cloned, which can convert pinoresinol to lariciresinol and consequently to secoisolariciresinol, and secoisolariciresinol dehydrogenase (SDH) gene, which can convert secoisolariciresinol to matairesinol. The total RNA of Podophyllum pleianthum Hance was used as the material for sdh cloning by using reverse transcriptase PCR (RT-PCR). The cDNA sequence of sdh which got from Podophyllum pleianthum Hance aligned with sdh cDNA sequence from Podophyllum peltatum. It reached to 98.1% identity. The alignment of amino acid sequence reached to 98.2%. The optimum conditions was used 0.01 mM IPTG inducting 9 hours at 25oC for expression of SDH in E. coli. The result showed a 34 kDa of protein in SDS-PAGE, the same size for sdh with a SDH-Histag design. The conversion of recombinant enzyme reaction was further analyzed by HPLC, the retention time (23.97 min) and the UV absorption spectrum matched with the characters of authentic matairesinol. It indicated that the cDNA sequence of sdh was cloned from Podophyllum pleianthum Hance and expressed in E.coli functionally. Meanwhile, cDNA of plr got from Podophyllum pleianthum Hance by using rapid amplification of cDNA ends PCR (RACE PCR) and RT-PCR, was aligned with plr cDNA sequence from Forsythia intermedia, and it reached to 68.9% identity. Alignment of amino acid sequence also reached to 75.2% identity and 85% similarity. Western blotting proved the expression of target protein PLR in E. coli. The results showed a 39 kDa of recombinant protein expressed in SDS-PAGE, the same size for sdh with a PLR-His tag design.