Hepatitis C virus (HCV) is a major cause of liver disease worldwide. HCV contains a positive-stranded RNA genome of 9.6 kilobases encodes a polyprotein of about 3000 amino acid residues. The polyprotein undergoes cellular and viral protease processing to generate structural and nonstructural proteins. Nonstructural protein 4B (NS4B) is a relatively hydrophobic 27 kDa protein of unknown function. NS4B has four transmembrane segments and has the ability to induce a tight structure formation as membranous web. It is proposed that HCV NS5B RNA polymerase forms replication complex with other nonstructural proteins at the membranous web. NS4B possesses GTPase activity. It contains a nucleotide binding motif (NBM) that mediates binding and hydrolysis of GTP previously demonstrated to be important for HCV replication. Substitutions at the conserved K-1846 with serine or arginine in the A motif (1840-GX1X2X3X4GK-1846) of NBM impaired GTP binding and hydrolysis, and resulted in inhibition of HCV RNA replication. Nevertheless, a cell culture adaptive mutant K1846T in which K-1846 was mutated to threonine enhances HCV RNA replication to 30 fold. In this study, NS4B and NS4B(K1846T) were detected in the cytoplasm of transfected cells and preferentially localized at the perinuclear region by immunofluorescence staining assay. To examine the NTPase activities of NS4B and NS4B(K1846T), GST-NS4B and GST-NS4B(K1846T) were expressed in E. coli, purified by glutathione Sepharose 4B, and cleaved to NS4B and NS4B(K1846T) by PreScission protease. HCV NS4B protein possesses both GTPase and ATPase activities. K1846T mutation decreased the ATPase activity of NS4B to 40%, but had little effect on GTPase activity. The results indicate that the lysine-1846 in the nucleotide binding motif is not absolutely required for the GTPase activity of NS4B. Different from previous studies, the results suggest that the adaptive mutant K1846T may promote HCV replication by mechanisms other than the GTPase activity of NS4B protein.