The hypocotyl sections, receptacle and filament of cabbage were used as explants cultured on MS medium supplemented with various plant growth regulators. It was demonstrated that the auxin had multiple effect on morphogenesis, varied with explant source, auxin type and concentration. For the hypocotyl sections, the picloram initially induced rhizogenesis, caulogenesis and callogenesis at the level of 0.01, 0.05 and 0.1 mg/l. respectively. In contrast, 2,4-D stimulated caulogenesis, rhizogenesis and callogenesis at 0.01, 0.05 and 0.1 mg/l. PAA ranging from 0.5 to 2.0 mg/l induced caulogenesis. The combination of 0.05 mg/l picloram and 0.5 mg/l BA showed additive effect on proliferation of adventitious buds through indirect caulogenesis. The frequency of adventitious buds of 'K-Y Cross', 'Spring Light' and 'Summer Summit' cultivars were about 80%, and obtained 28 to 31 shoots per explant within smooth. The regeneration frequency of 'Chung-Kan No.11' was highest up to 100%. It was shown that higher picloram (0.1 mg/l) decreased the frequency of bud formation. Addition of AgNO3 and STS respectively enhanced regeneration to 81.2% and 76.2% in 'K-Y Cross.' The ethylene inhibitors were less effective in 'Spring Light' for bud regeneration. Interpreting that the inhibition of higher auxin concentration on adventitious bud formation might be mediated through ethylene evocation. To the cultured of receptacle tissues, us morphogenetic event as observed with austin alone. When a combination of 0.05 mg/l picloram and 0.5 mg/l BA were used, more than 95% of explants from 'K-Y Cross' and 'Spring Light' insisted bud proliferation. The anatomical feature in sole picloram induction of caulogenesis was initiated from the distal end of hypocotyl sections. The neighbor tissue of vascular bundle dedifferentiated into meristemoids, then regenerated adventitious buds 14 days after culture. In combination of picloram and BA, emitting cells from the neighbor tissue of vascular bundle differentiated iota discreted meristematic center and primary buds. Multiple shoot proliferated from the periphery of meristematic bells or primary buds. In culturing receptacle tissue, the caulogenesis mainly derived from the pre-existing undeveloped stamen primodium, that perform as meristematic structure body. The internal bud primordium initiated as early as 5 days after culture. Thereafter, the based of raising primary bud and callus-mediated meristemoids proliferated numerously adventitious buds.