The molecular farming may produce pharmaceutically valuable protein or enzymes of the industrial application. The establishment of gene transformation contribute to develop molecular breeding and molecular farming. In this study, the expression system using Agrobacterium tumefaciens-mediated transformation (ATMT) was developed. A. tumefaciens inserts the T-DNA which is a portion of Ti-plasmid into the genome DNA randomly during infecting host. It could make the target gene more stable and enhance protein analysis. The expression plasmids were constructed to harbor homologous glyceraldehyde-3-phosphate (gpd) promoter from Hypsizygus marmoreus variant (Hmv), Escherichia coli hygromycin B phosphotransferase gene (hph) as the selectable marker and enhanced green fluorescent protein gene (egfp) as reporter gene. A. tumefaciens carrying these plasmids were cocultivated with vegetative mycelia, modified mycelia pellets (MMP) of Hmv for 3~6 days, respectively. The transformation efficiency was 1 transformant per mg dry weight of mycelia and about 30~40% with MMP. The heterologous gpd promoters from Agaricus bisporous and Flammulina velutipes expressed egfp gene successfully in Hmv. The western blotting analysis revealed the EGFP was expressed indeed. From the ELISA quantification analysis, the egfp expressed by Hmv promoter could reach to 27.4 ng per gram dry weight of mycelia, which was higher than by A. bisporus and F. velutipes. This study show the homologous Hmv gpd promoter was more efficient for egfp expression in Hmv than heterologous promoter. In this study, we cloned the succinate dehydrogenase gene (sdi1) from Hmv and introduced a point mutation that confers carboxin resistance into it. After transfer the recombinant plasmid into Hmv by ATMT, we could get the transformants which confers homologous selectable resistance.