The evidence of proteins at the yeast cell surface that lack N-terminal signal peptides was initially provided by morphological, biochemical and genetic studies. The existence of many such proteins has subsequently been demonstrated by proteomic approaches. In Candida albicans, the gene encoding enolase is named CaENO1. Enolase is an enzyme of glycolysis and gluconeogenesis as well as major cell-surface antigen, which binds host plasmin and plasminogen. It is immunoprotective, phagocytosis, biofilm-regulated, and farnesol-down regulated. Enolase is detected on the cell surface even in the culture medium, but the mechanism of secretion is still unknown. My study was focused on identifying the critical region of CaENO1 for secretion. First step is to test whether CaENO1 can be expressed in Saccharomyces cerevisiae, CaENO1 was tagged with HA3HIS6 and EGFP, respectively for detecting the target protein. Second is to further analysis the protein secretion. For determining which region is critical, the CaENO1 was truncated for obtaining the constructs with different fragments 1-150 bp, 1-279, 1-387, 1-450, 1-510, 1-900, 280-1320, 388-1320, 451-1320, 901-1320, 451-901 of CaENO1 and negative control EGFP only construct, and then analyzed for the secretion of truncated CaENO1-EGFP protein with western blot. According to the result of western blot, only full length CaENO1 can lead the tagged protein outside the cell. Using confocal laser scanning microscopy, the eno-EGFPp was localized in the cytoplasm but not in the cell membrane or cell wall.the. S. cerevisiae cell seems not recognize the eno-EGFPp as a cell wall protein in this study.