Some previous studies have showed that IPAF (immunodulatory protein of Anoectochilus formosamus) could activate mouse macrophages through TLR4 pathway and directly stimulated the proliferation of B lymphocytes without the help from T lymphocytes. These results suggested that IPAF might be a type 1 thymus-independent antigen. The objective of this study was to clone the cDNA encoding IPAF. First, we used the N-terminal amino acid sequence assay to acquire the N-terminal amino acid sequence of IPAF, ASSLGTGGTLRNN, and designed the IPAF degenerated specificity primers based on the N-terminal amino acid sequence. We then used 3’-rapid amplification of cDNA ends (RACE) and 5’ RACE PCR to generate the full-length IPAF cDNA. We then searched in NCBI database for similar nucleotide and amino acid sequences. The result showed that the full-length IPAF cDNA was 654-bp, and ORF was 474-bp, respectively. The protein encoded consisted of 158 amino acid residues. It was predicted that IPAF contained a putative residual signal peptide of 25 residues by the SignalP prediction assay. The molecular weight and pI value of amino acid sequence from residue 26 to 158 as predicted by the compute pI/Mw tool assay were 14312.02 Da and 9.62 respectively, which were similar to the native IPAF. The result of cross searching in NCBI database showed that the amino acid sequence of IPAF was highly similar to that of Epipactis helleborine lectin. A cDNA encoding mature IPAF was cloned into pET30 plasmid vector and expressed in Escherichia coli.. A fusion protein could then be induced by 1mM IPTG for six hours. This study suggested that the amino acid sequence of IPAF provided supportive information for future investigation regarding the structure, active domain and functional analysis of IPAF.