关键词: 广西巴马小型猪, 卵泡抑素, 克隆, 原核表达

Abstract: In this study,the total RNA was isolated from Guangxi Bama mini-pig ovary tissue with RNA_(watson) extraction kit.The complementary DNA(cDNA) encoding Follistatin protein was ampilified by the reverse transcription polymerase chain reaction(RT-PCR) method and a pair of differential primers.The amplified cDNA fragment was inserted into pMD18-T vector.The recombined vectors were verified through the sequence survey.The results showed that the cloned Follistatin cDNA was highly homologous with the reported nucleotide encoding swine Follistatin in GenBank(99.4%).Meanwhile,the identified Follistatin cDNA was inserted in the multiple cloning sites of plasmid pET 32a+ to construct prokaryotic expression vector,the latter was transformed into the E.coli.BL_(21) induced by IPTG.Then a fusion protein was obtained(about 58.4 ku) in SDS-PAGE and Western blotting.These results showed that the Follistatin cDNA was expressed in prokaryotic cells.

Key words: Guangxi Bama minipig, Follistatin, Cloning, Prokaryotic expression