Abstract In order to understand the characteristics of gibberellin biosynthesis genes encoding GA 20-oxidase and GA 2-oxidase in Phalaenopsis, homologous DNA fragments from Arabidopsis thaliana were used as probes to screen Phalaenopsis cDNA library. Nucleotide sequence analysis revealed that pPhGA20ox-1-50 cDNA, designatedd as PhGA20ox1, was 1478 bp in length, encodes a polypeptide of 372 amino acid residues with a calculated molecular weight of 41.9 kD and isoelectric point 5.96. The deduced amino acid sequence of PhGA20ox1 contains conserved domain LPWKET, NYYPXCXXP and three histidines, which are considered to be involved in the binding of substrate GA, cosubstrate 2-oxoglutarate and Fe2+, respectively. PhGA20ox1 mRNA was expressed in roots, flower stem, leaves, flowers, buds and flower petiole of Phalaenopsis, especially in roots and leaves. Gene expression of PhGA20ox1 was induced by H2O2 with a highest transcript level induction at 50 mM. Moreover, expression of PhGA20ox1 did not respond to UV irradiation. One of the GA 2-oxidase cDNA, pPhGA2ox-3-79, has also been cloned from Phalaenopsis. This cDNA was 689 bp in length, and the deduced polypeptide of pPhGA2ox-3-79 cDNA lacked the N- and C- terminus as compared to other GA 2-oxidase amino acid sequences. To obtain the corresponding gene, pPhGA2ox-3-79 cDNA was used as the probe to screen genomic library of Phalaenopsis. Genomic clone λphg1-1 containing PhGA2ox1 was sequenced and characterized. The sequence analysis revealed that PhGA2ox1 was 3841 bp in length with a 954 bp open reading frame and encoding a 317 amino acid polypeptide. This gene contains two exons and one intron of 1488 bp. The deduced amino acids contained the histidine and aspartic acid residues which were found to be involved in the binding of Fe2+. No PhGA2ox1 transcripts were detected in Nothern analysis of different organs in Phalaenopsis, and PhGA2ox1 expression was not induced by UV. However, the PhGA2ox1 was expressed in Phalaenopsis upon exposure to 50 mM of H2O2.