The purpose of this paper is to investigate the differential responses of flower opening to ethylene in two cut rose cultivars, ‘Samantha’, whose opening process is promoted, and ‘Kardinal’, whose opening process is inhibited by ethylene. Ethylene production and 1- aminocyclopropane-1-carboxylate (ACC) synthase and oxidase activities were determined first. After ethylene treatment, ethylene production, ACC synthase (ACS) and ACC oxidase (ACO) activities in petals increased and peaked at the earlier stage (stage 3) in ‘Samantha’, and they were much more dramatically enhanced and peaked at the later stage (stage 4) in ‘Kardinal’ than control during vasing. cDNA fragments of three Rh-ACSs and one Rh- ACO genes were cloned and designated as Rh-ACS1, Rh-ACS2, Rh-ACS3 and Rh-ACO1 respectively. Northern blotting analysis revealed that, among three genes of ACS, ethylene-in- duced expression patterns of Rh-ACS3 gene corresponded to ACS activity and ethylene production in both cultivars. A more dramatic accumulation of Rh-ACS3 mRNA was induced by ethylene in ‘Kardinal’ than that of ‘Samantha’. As an ethylene action inhibitor, STS at concentration of 0.2 mmol/L generally inhib-ited the expression of Rh-ACSs and Rh-ACO in both cultivars, although it induced the expression of Rh-ACS3 transiently in ‘Kardinal’. Our results suggests that ‘Kardinal’ is more sensitive to ethylene than ‘Samantha’; and the changes of Rh-ACS3 expression caused by ethylene might be related to the acceleration of flower opening in ‘Samantha’ and the inhibition in ‘Kardinal’. Additional results indicated that three Rh-ACSs genes were differentially associated with flower opening and senescence as well as wounding. The purpose of this paper is to investigate the differential responses of flower opening to ethylene in two cut rose cultivars, ’Samantha’, whose opening process is promoted, and ’Kardinal’, whose opening process is inhibited by ethylene. Ethylene production and 1- After ethylene treatment, ethylene production, ACC synthase (ACS) and ACC oxidase (ACO) activities in petals increased and peaked at the earlier stage (stage 3) in ’ Samantha ’, and they were much more dramatically enhanced and peaked at the later stage (stage 4) in’ Kardinal ’than control during vasing. CDNA fragments of three Rh-ACSs and one Rh- ACO genes were cloned and designated as Rh- ACS1 , Rh-ACS2, Rh-ACS3 and Rh-ACO1. Northern blotting analysis revealed that, among three genes of ACS, ethylene-in- duced expression patterns of Rh-ACS3 were genetically modified to ACS activity and ethylene production in both c A more acute accumulation of Rh-ACS3 mRNA was induced by ethylene in ’Kardinal’ than that of ’Samantha’. As an ethylene action inhibitor, STS at concentration of 0.2 mmol / L generally inhibits it and Rh-ACO in both cultivars, although it induced the expression of Rh-ACS3 transiently in ’Kardinal’. Our results suggests that ’Kardinal’ is more sensitive to ethylene than ’Samantha’; and the changes of Rh-ACS3 expression caused by ethylene might be related to the acceleration of flower opening in ’Samantha’ and the inhibition in ’Kardinal’. Additional results indicated that the three Rh-ACSs genes were differentially associated with flower opening and senescence as well as wounding.