Objective:To clone, express and purify a putative parasitic nematode specific protein of Setaria digitata (S. digitata), filarial nematode that infects livestock and cause significant economic losses inFarEast andAsia to be used for structural and functional analyses. Methods:To characterize uncharacterized gene ofS. digitata(SDUG), the herterologous expression ofSDUG was carried out in the pET [cloned into pET45b(+)] expression system initially and co-expression ofSDUG using chaperone plasmids pG-KJE8, pGro7, pKJE7, pG-Tf2 and pTf16 containing chaperone proteins of dnaK-dnaJ-grpE-groES-gro-E, groES-groEL, dnaK-dnaJ-grpE, groES-groEL-tig, and tig respectively, was carried out subsequently.Results:Expression ofSDUG was seen whenEscherichia coli strainBL21(DE3) is used, while concentrating protein largely into the insoluble fraction.The co-expression ofSDUG using chaperone plasmid mediated system indicated a significant increase of the protein in the soluble fraction.Of the chaperon plasmid sets, the highest amount of recombinantSDUP in the soluble fraction was seen when pGro7 was used in the presence of 2 mg/mLL-arabinose and0.6MIPTG concentration in the culture medium and for3 h of incubation at the temperature of28 ℃.RecombinantSDUG was purified both from soluble and insoluble fractions usingNi affinity chromatography.SDS-PAGE and west blot analyses of these proteins revealed a single band having expected size of ~24 kDa.Conclusions:SDUG seems to be more aggregate-prone and hydrophobic in nature and such protein can make soluble by correct selecting the inducer concentrations and induction temperature and its duration.