An Agrobacterium-mediated plant transformation system was developed for the commercial banana(Musa spp. AAA group) 'Pei Chiao' by using embryogenic calli induced from young male inflorescence. Theembryogenic calli were co-cultivated with Agrobacterium tumefaciens strain LBA4404, harbouring thebinary plasmid pBI121. The vector carried NPTII (neomycin phosphotransferase) and GUS (β-glucuronidase) genes in the T-DNA. Putatively transformed calli were produced on a selection medium supplemented with 50 mg•L^(-1) geneticin (G418). The primary antibiotic-resistant calli were subsequently transferred to theselection medium containing 110 mg•L^(-1) G418. After selective cultures, the callus lines (putativehomogenous GUS-expression) were transferred to MS medium containing 0.05 mg•L-1 zeatin, 0.2 mg•L^(-1) 2iP, 0.1 mg•L^(-1) kinetin, 0.2 mg•L^(-1)NAA and 110 mg•L^(-1) G418 for somatic embryogenesis. Finally, theantibiotic-resistant somatic embryos were transferred to MS medium containing 1 mg•L^(-1) BA, 0.1 mg•L^(-1)GA3 and 30 mg•L^(-1) sucrose for plant regeneration. Stable integration and expression of the transgenes wereconfirmed by GUS assay, polymerase chain reaction (PCR), and genomic Southern hybridization analyses.