Immature embryos of soap berry (Sapindus mukorossi Gaerm.) in the National Taiwan University campus were collected for callus induction via tissue culture techniques to study on the effects of different factors on somatic embryogenesis. Techniques of cell suspension culture and embryogenesis were employed to establish an economic, stable and effective system for micropropagation of seedling and to facilitate selection and breeding of superior strains of soap berry. While immature soap berry embryos being cultured in WPM media, addition of 0.1mg/L NAA could promote rooting and budding. Callus could be induced after 4 weeks by cutted grown hypocotyls sub-cultured on WPM medium with 0.3 mg/L kinetin. In this work, the optimal cultivation condition for somatic embryogenesis induction of S. mukorossi was made by sub-culturing 0.5 cm × 0.5 cm × 0.5 cm callus clump on WPM medium with 2% sucrose, double NH4+content, 0.1 mg/L NAA and 0.05mg/L TDZ, under 28μEm-2s-1 average light intensity, 16 hrs photoperiod for 8 weeks. Then, optimal somatic embryogenesis induction ratio could be achieved. In order to induce secondary somatic embryo after embryogenesis, 0.1 ~ 0.5 mg/L GA3 could be added in medium to promote secondary somatic embryogenesis. To promote seedling, concentration of GA3 could be increased to 2 mg/L in medium to promote the embryo maturation and the ratio of emblings conversion. In the aspect of cell suspension culture, using callus induced from soap nut hypocotyls of as starting materials, some cell microsphere and cell with dense cytoplasm gradually appeared after sub-culturing for 2 ~ 4 months. Hence, longer sub-culturing time could be required to obtain extricated embryogenic callus.