Cellulose, hemicellulose, and lignin are most abundant macromolecules in nature. Lignin is hardest to be degraded for its complex constitutions. There are three enzymes have the ability to degrade lignin: laccase (1.10.3.2), manganese peroxidase (1.11.1.13), and lignin peroxidase (1.11.1.14). Whitr-rot fungi, such as Ganoderma spp., can degrade lignin. In this study, gene family, characteristics, and heterologous expression of laccase genes from Ganoderma spp. are discussed. The specific primers according to laccase conserved copper-binding regions used to amplify the laccase genes in the eleven strains of Ganoderma spp. There are 26 partial laccase genes were cloned in this study. The result shows that there are at least two laccase genes in each strain. The phylogenetic relationship shows that laccases from G. spp can be divided into three groups and each group has their own introns which might suggest that these three groups have different evolutionary relationship. The third group might exist before the speciation for G. spp and Trametes. The full length laccase gene of RZ.lac4 、0814.lac1 、1109.lac1 from G. lucidum RZ、G. tsugae 1109、G. fornicatum 0814 were 2121bp, 2019bp, and 2110bp, and there are 9 introns in each sequence. Laccase cDNA of RZ.lac4 、0814.lac1 、1109.lac1 were cloned and encodes for proteins with 520, 521, and 521 amino acids, including a 21-residue secrection signal peptide for each protein. Phenylalnine in additional residue 10 amino acids downstream of the conserved cysteine of each encoding protein shows that these proteins belong to class 3 laccase and may have high redox potential of the cupric ion. 5’ Genome walking of RZ.lac4 from G. lucidum RZ shows that TATA box, CAAT box, The Mental-responsive elements (MREs) and stress-responsive promoter element (STRE) exist in the promoter region of RZ.lac4. The Mental-responsive elements and stress-responsive promoter element found in the promoter of RZ.lac4 suggest that RZ.lac4 might be regulated by mentals. The cloned cDNA were subcloned to pPICZ vectors and expressed in Pichia pastoris KM71 under the control of the AOX1 promoter. The transformants were found to secrete active recombinant enzymes after induction with methanol. The optimal temperature of the recombinant proteins, reRZ.lac4, re0814.lac1, re1109.lac1, are 55, 55-75, and 65 . The ℃ optimal pH for the recombinant proteins is 3.0. The transformants were incubated in BMMHY medium at 30℃ with 0.5% MeOH at 250rpm each day. The laccase activities for reRZ.lac4, re0814.lac1, re1109.lac1 were 1.13U/ml、5.9U/ml、6.6U/ml，and the specific activities were 32U/mg、 90.2U/mg、81.7U/mg measured at optimal pH and temperature with ABTS as substrate. These three recombinant proteins were incubated in 30℃ for 24 hours, and all of them retained activities above 90%. Re1109.lac1 was incubated in 55℃and still retained almost 100% activity which shows that the protein has good thermostability. The culture medium of Re0814.lac1 was added to different pH buffer at room temperature for 24h, all of them still retained above 90% activity. This infers that re0814.lac1 might have good pH stability.