The purpose of this study is to establish an efficient, stable and practical gene transfer system for cabbage (Brassica oleracea L. var. capitata L). The plasmid pRT99gus containing the reporter gene GUS encoding β-glucuronidase and selectable marker NPTII gene was introduced by injection into placenta tissue of recipient. The cultivated cabbage KYcross variety was used as recipient plant. By spraying kanamycin (100mg/l) on cabbage plant, 34 out of 137 T1 plants showed resistant to kanamycin. Based on DNA blot hybridization analysis, 29 out of 137 showed positive signals. Among them, 13 plants showed both resistant to kanamycin and hybridization signal. After selfing, the progeny of the T1 plants was farther assessed for the transmission of integrative transformation. The proportion of the progeny (T2) showing positive hybridization signals was 3/4 for one of the T1 plants. This result suggests that exogenous DNA can be integrated into cabbage genome and inherited lathe next generation. Thus, gene transfer through pollen tuba pathway was proved to be feasible on the molecular level.