Expression of selectable marker genes allows scientists to identify and isolate the transgenic cells. Once the transgenic plant has been generated, marker gene generally no longer serves an essential purpose. Furthermore, the propagation and development of transgenic cells will be retarded if the antibiotic or herbicide remains in the growth medium. Besides, it is concerned by publics about biosafety of antibiotic and herbicide resistance genes in transgenic plants. We have developed four different constructs under the control of the promoter PR-1afor inducible transposon systems as marker-free strategy and theses constructs were transformed into Phalaenopsis calli and tobacco plants. Transgenic plants were treated with 3 mM salicylic acid for 5 days to eliminate marker genes. Four patterns of transposition have been identified base on sequence analysis. Residual DNA sequences of 35 - 128 bp were fused as footprints after excision of the transposon. Southern analysis confirmed further that the herbicide resistance geneEPSPS,had been removed together with the transposition.