Abstract Ganoderma membrane in homogeneous conditions for wound healing and absortive reparing of soft tissues was investigated as well as the structure of Ganoderma residues was indentified in present study. Ganoderma residues after removing the triterpenes and polysaccharide were used for the treatment with several concentrations of NaOH, then the treated residues were water-washed to neutral pH. The NaOH treated residues were bleached with various concentrations of NaClO3 before another water-washed to remove pigment. Washing was lasted until the AgNO3 indicated negative reaction in the leach. After that, bleached Ganoderma residues were lyophilized for 3 days and 8% of the dried samples were dissolved in , a binary solvent, 6% LiCl/DMAc system for 3 days. The dissolved systems were put subsequently in ethanol for 120 seconds, then in acetone for 15 seconds, and finally in water for 60 seconds. The membranes were water-washed for 24 hours and then casted on Teflon papers to allow on drying in room temperature to produce a transparent membrane. Chemical structrure of GANOCHITIN was analysed by NMR, IR, GC/MASS to identify the Chitin structure with a cross-linked b-glucan at C-3 position. The strength measured by DMA indicated that GANOCHITIN has a stronger tensile. MTT assay of GANOCHITIN showed no cytotoxicity to cell line. Analysis DSC and X-ray indicated that degree of crystallinity increased slightly after dissoling and casting. The viscosity of the dissolving samples was measured to compare molecular weight with another by viscosity meter. The result of the present study could be useful for the optimation for large scale production of GANOCHITIN and further test in vivo.