Mature human erythropoietin gene was amplified from EPO cDNA by PCR methods. The PCR product was cloned into pUC18 plasmid at Sma I site, then precisely engineered into a intermidiate vector pSK43SB which were digested with Hind III, Mung bean nuclease, and Sal I. Then degest pSK43SB-EPO plasmid with EcoR I and Cla I, the EC fragment with an alpha-factor leading sequence, EPO gene and CYC1 terminater were produced. It was then cloned into a typical high efficiency episomal expression vector YEpHC8. Human EPO protein with highly mannose glycosylated was identified by Western blot methods in both secreted and in cells proteins. N-Glycosidase F digested secreted EPO can produce 20,000 EPO without N-glycosylation similar with that produced in cells.