关键词: 日本血吸虫, 嘌呤代谢, 腺苷脱氨酶

Abstract: Objective To clone and express a new protein adenosine deaminase of Schistosoma japonicum (SjADA). Method Specific primers were designed according to the EST sequence and used for amplification of the encoding sequence from the cDNA clone containing SjADA. The gene was sub-cloned into pET32 plasmid and expressed in E.coli BL31(DE) pLys strain and the recombinant proteins were purified by chelating sepharose FF. The structure and phylifunctions of this protein were analyzed by MrBayes and GeneAtlas. Result The full length sequence of SjADA gene was obtained and the recombinant protein was cloned, expressed and purified successfully. The bioinformatics analysis showed that the identity of SjADA and SmADA gene sequence was only 25% and they belonged to different subfamily. The structure of SjADA had 41% identity with it’s PDB template 1A4M. Conclusion The recombinant protein of SjADA has been obtained. The purine salvage pathway of S. japonicum may be different with that of S.mansoni.

Key words: Schistosoma japonicum, Purine metabolism, ADA