The intestinal protozoan Giardia lamblia is a water-borne flagellated parasite. It causes non-bacterial diarrheal disease, also known as giardiasis, throughout the world. The life cycle stages of G.lamblia is composed of cyst and trophozoite. Cysts are the infected form and resistant to environment, trophozoites are the active form which colonizes in the small intestine. Encystation, a process of cell differentiation from trophozoites to cysts, is necessary for transmission between hosts. During encystation, transcription factors Myb2 and E2F1 up-regulate genes encoding cyst wall proteins (cwps).The initiation of encystation is associated with cell cycle progression, so we attempt to identify the role of cyclin-dependent kinases (Cdks), critical cell cycle regulators, in encystation. We have found a putative cdk gene in G. lamblia database. Amino acid sequence analysis showed the Cdk homologue is similar to human Cdk1 and it contains a PSTAIRE-like motif, PGTAIRE, so we named it Giardia Cdk1. We found that mRNA and protein levels of Cdk1 were increased during encystation. Overexpression of Cdk1 resulted in increasing ability of cyst formation. Moreover, using immunoprecipitation- kinase assay, we also found that Cdk1 was able to phosphorylate Myb2 and E2F1 proteins. We constructed a set of mutants including mutation in PGTAIRE motif that may be involved in cyclin-binding which named Cdk1-m1, the aspartic acid at residue 159 that may be involved in ATP-binding and deletion of a large segment of kinase domain which named Cdk1-m2 and Cdk1-m3, respectively. Compared to wild type Cdk1, mutations of these important regions of Cdk1 leaded to decreased the levels of cwp genes expression, kinase activity, and cyst formation. The results suggest that Cdk1 is a positive regulator in encystation of G. lamblia.