Phaius tankervilliae is an indigenous orchid of Taiwan. Owing to be an almost extinct species, the plant needs to be protected extremely. Virus-like mosaic symptoms were observed on the leaves of P. tankervilliae which were found in mountain area of Chung-ho, Taipei County. Systemic symptom and chlorotic lesions appeared when we mechanically inoculated the plant saps onto the leaves of Nicotiana benthamiana and Chenopodium quinoa, respectively. After three successive single lesion isolations in C. quinoa, one virus isolate was obtained and named PT. The host range test of PT isolate was performed. We observed the filamentous virus particles with length of 750 nm in crude plant extract via the transmission electron microscope (TEM). Indirect ELISA test showed that the originally infected and PT-inoculated plants reacted with anti-potyvirus monoclonal antibody positively. Furthermore, RT-PCR was performed by using degenerate primers for potyviruses. A 1.8-kb fragment was amplified and cloned. The sequence of the fragment was compared with the NCBI GenBank database. The result indicated that the 1.8-kb fragment of PT isolate containing the 3’-terminal region of potyvirus including partial NIb gene, CP gene and 3’ untranslated region (UTR). Moreover, it had 97% nucleotide identity with Bean yellow mosaic virus (BYMV). Therefore, the virus obtained from P. tankervilliae is an isolate of BYMV, and designated as BYMV-PT isolate. RT-PCR and 5’RACE techniques were employed to analyze the remaining sequence of BYMV-PT by utilizing potyvirus degenerate primers and BYMV specific primers. After cloning, sequencing and analysis, the genomic sequence of BYMV-PT has 9547 nucleotides in length excluding poly(A) tail. Besides the 205-nt 5’UTR and 174-nt 3’UTR, there is one large open reading frame which encodes a polyprotein of 3046 amino acids with an M(r) of 347 kDa. According to the proteinase cleavage sites, the polyprotein can be processed into P1, HC-Pro, P3, 6K1 and 6K2, CI, NIa-VPg, NIA-Pro, NIb, and CP. Through the whole genome comparisons of BYMV-PT with other 44 potyviruses, BYMV isolates clustered together, and the most closely related virus to BYMV is Clover yellow mosaic virus (ClYVV). In order to study the function of virus genes during infection process, we used positional cloning and RT-PCR amplification to construct BYMV-PT full-length cDNA clone and acquired 23 clones with T7 promoter. The biological activity test of the cDNA clones of BYMV-PT is still going on. By back inoculation of BYMV-PT to healthy P. tankervilliae, the ELISA value was positive for the inoculated plants 7 days after inoculation. It demonstrated that P. tankervilliae could be infected by BYMV-PT. However, no obvious symptom was observed yet.