For the production of the recombinant human interferon-gamma(rhIFN-${gamma}$) in Escherichia coli, human glucagon and ferritin heavy chain were used as fusion partners. Even though rhIFN-${gamma}$ is expressed as an inclusion body form in E. coli because of strong hydrophobicity of itself, over 50% of fused rhIFN-${gamma}$ was expressed as soluble form in E. coli $Origami^{TM}$(DE3) harboring pT7FH(HE)-IFN-${gamma}$ which encodes ferritin heavy chain-fused rhIFN-${gamma}$. In the case of using glucagon-ferritin heavy chain hybrid mutant as a fusion partner, 6X His-tag was additionally introduced to N-terminus of GFHM(HE)-IFN-${gamma}$ for enhancing purification yields of rhIFN-${gamma}$. Fusion protein HGFHM(HE)-IFN-${gamma}$ with two 6X His-tag was more effectively bound to Ni-NTA agarose bead than GFHM(HE)-IFN-${gamma}$ with a 6X His-tag. rhIFN-${gamma}$ was completely purified from enterokinase-treated HGFHM(HE)-IFN-${gamma}$ by Ni-NTA affinity column. For high-level production of rhIFN-${gamma}$, glucose was used as the sole carbon source with simple exponential feeding rate($2.4{sim}7.2g/h$) in fed-batch process. The effective lactose concentration for the expression of the rhIFN-${gamma}$ was $10{sim}20mM$. Under the fed-batch culture conditions, rhIFN-${gamma}$ production yield reached 11 g DCW/L for 6 hours after lactose induction.