Pleione formosana Hayata is a Taiwan-native deciduous orchid species suitable for transportation to meet European and Japanese market`s demand. Though cultivars have been developed but sales were limited due to low propagation efficiency. This study aimed to determine suitable conditions for mass propagation of P. formosana ‘Mei Snow’ and ‘Feng Star’ by somatic embryogenesis or multiple shooting. Bud from cold stored P. formosana corms were taken as explants, and cultured on mediums containing various plant growth regulator combinations. Light intensity and quality during in vitro and ex vitro acclimatization were tested to increase growth and ex vitro survival. The effect of in vitro cultured duration on ex vitro growth was also studied. The fourth bud on P. formosana corms after cold storage at 0, 2, 4, 6, 8, 10, 12, and 15oC for 4, 6, and 8 weeks were taken as explants. The fourth bud explants were cultured on 1/2 Murashige & Skoog (MS) medium containing 20 g•L-1 sucrose, 4 g•L-1 gelrite, 0.15 mg∙L-1 NAA (naphthalene acetic acid), and 0.2 mg∙L-1 BA (benzyl adenine purine). Those stored at 2-8oC for 6 weeks showed higher multiplication rate when cultured after 24 weeks. Apical bud, the fourth bud, and the fifth bud of P. formosana ‘Mei Snow’ stored at 5oC for 6 weeks were taken as explants. Only the fourth bud and the fifth bud explants were able to regenerate after cultured on 1/2 MS medium containing 20 g•L-1 sucrose, 3 g•L-1 Tryptone, 4 g•L-1 gelrite, and 2 g•L-1 activated charcoal. Direct somatic embryo were induced when the fourth and the fifth bud explants were cultured on 1/2 MS medium supplemented with 1.2, 2.4 mg•L-1 Dicamba or 1.1, 2.2 mg•L-1 Picloram and 0.2 mg•L-1 BA. Multiple shooting regenerated from the fourth bud culture were divided as secondary explants, and cultured for 8 weeks on 1/2 MS medium supplemented with NAA and BA combinations. Results showed those cultured on 0.2 mg•L-1 NAA combined 0.4 mg•L-1 BA induced more somatic embryos, with growth phase similar to seed-develop plantlets. Secondary somatic embryos were induced from surface of primary somatic embryos after subcultured to 1/2 MS medium containing 0, 0.2, and 0.4 mg•L-1 NAA and BA combinations. Secondary somatic embryos shared similar growth stage with primary somatic embryos. Somatic embryos tended to develop plantlets with increasing NAA concentration. Anatomical reservation showed that plantlets developed from somatic embryo had independent isolated vascular bundle. Leaf tip, leaf base, and corm slice from in vitro plantlets were also taken as explants, but only corm slices with buds could regenerate to plantlets. More somatic embryos were induced from those cultured on 1/2 MS medium supplemented with 0.2 mg∙L-1 2, 4-D or NAA combined with 0.2 mg∙L-1 BA. Plantlets cultured with LED (light emitting diode) white light (19% red + 52% green + 29% blue) had more buds, fresh weight, corm diameter, and leaf length than those cultured with LED red, LED blue, LED red plus blue light, and fluorescent lamp. Suitable light intensity for in vitro culture was 30 μmol•m-2•s-1 PPF. Ex vitro plantlets were acclimatized under 30, 60, and 90 μmol•m-2•s-1 PPF for 2 weeks. Results showed that plantlet acclimatized under 30 μmol•m-2•s-1 showed higher Fv/Fm value and net photosynthesis, but those acclimatized under 60 and 90 μmol•m-2•s-1 had higher survival rate and better growth after transplanting. En vitro plantlets were also acclimatized under various light quality at 60 μmol•m-2•s-1 for 3 weeks. Results showed that plantlets under LED white light had higher net photosynthesis, survival percentage, and more growth after transplanting. Plantlets cultured in vitro after 8, 12, and 16 weeks were transplanted and acclimatized under 60 μmol•m-2•s-1 for 3 weeks. Results showed that higher survival rate, fresh weight, corm diameter, and root number were recorded in plantlets cultured for 12 and 16 weeks then that cultured for 8 weeks.