The non-structural protein 5A (NS5A) is a critical hepatitis C virus (HCV) protein required for the viral life cycle. It is a phosphoprotein with two phosphorylation states: hypo- and hyper-phosphorylated NS5A that appear at 56 (p56) and 58 (p58) kDa on immunoblots. Numerous genetic mutations followed by functional assays have pinpointed several serine residues that are critical for NS5A hyper-phosphorylation and for viral replication ability, indicating a role of hyper-phosphorylated NS5A in HCV replication. The functions of hypo-phosphorylated NS5A are less understood. My thesis work aimed to distinguish the proteins that bound to hypo- vs. hyper-phosphorylated NS5A using co-immunoprecipitation followed by LC-MS/MS analysis. We have previously generated a hyper-phosphorylation specific antibody that specifically detected hyper-phosphorylated NS5A. Here, we generated a hypo-phosphorylation specific antibody that detected only hypo-phosphorylated NS5A. Using stimulated-emission depletion based super resolution microscopy, the hypo- and hyper-phosphorylated NS5A were found in discrete intracellular localization, suggesting that these two phosphorylation forms of NS5A may have discrete functions. Co-immunoprecipitation followed by label-free quantitative proteomics identified proteins that bound to hypo- vs. hyper-phosphorylated NS5A. A total of 534 proteins were quantified in two replicates. Among the quantified proteins, 104 proteins showed favorable interacting with hyper-phosphorylated NS5A and 14 proteins showed favorable interacting with hypo-phosphorylated NS5A. DAVID Gene Ontology term analysis of the proteins bound to hyper-phosphorylated NS5A revealed terms predominantly associated with cell migration and RNA replication.