Human P-selectin glycoprotein ligand-1 (PSGL-1) is a 43 kDa glycoprotein and common found on leukocytes and endothelial cells. PSGL-1 needs two important post-translational modifications to regulate the binding affinity with cell adhesion molecules - Selectins. One is Tyrosine O-sulfation through tyrosylprotein sulfotransferase (TPST, EC 2.8.2.20) transferred sulfuryl groups to Tyr-46、Tyr-48、Tyr-51 three potential positions of PSGL-1 N-terminal; the other one is Glycosylation that added Sialyl Lewis x tetrasaccharide (sLex) to O-linked glycans of PSGL-1 Thr-57 position. According to previous studies, such tyrosine-sulfated proteins participate in many physiological processes of inflammatory and coagulation response and has been identified as a key marker to mediate protein-protein interaction with Enterovirus (EV71) capsid protein VP1 invasion. However, there are still many questions about the stability and sulfation degree of sulfated proteins, due to the difficulty of sulfated proteins purification. Combination of PAPSS-TPST and PST-TPST sulfation coupled enzyme assay that has been developed in our laboratory by traditional biochemical methods, i.e. The native gel electrophoresis system could quickly be to analyze and identify the sulfated GST PSGL-1, and the GST PSGL-1 Y51K and GST PSGL-1 Y51E with different Tyr-51 site residue’s charges as a control. Overall, the purification methods, to develope sulfation coupled enzyme assay and gel electrophoresis system, the post-translational modification research were described in detail in this thesis.