Baculovirus, H cunea nuclear polyhedrosis virus(NPV) DNA genome was digested with EcoR I endonuclease and transformation in E. coli JM 83 using the plasmid vector pUC8. Four EcoR I site of plasmid vector pUC8 and identified by digestion of the recombient DNAs with EcoR I enzyme. The recombinents are named as LK-l, LK-2, LK-3 and LK-4. The total cell polypeptides of the recombinents and E. coli JM 83 were analyzed on the SDS-PAGE. Recombinents, LK-l, LK-2, and LK - 3 were appeared one new band as comparison with polypeptide bands of E. coli JM 83 cell. The molecular weight of new band was approximately 47.5Kd. The DNA genome was digested with Kpn Ⅰ, Pst Ⅰ, Pvu Ⅱ and Xho Ⅰ restriction endonucleases and hybridized with (a^(32)p)-labelled AcNPV polyhedrin gene cDNA. The probe DNA hybredized to Kpn Ⅰ-A, Pst Ⅰ- F, Pvu Ⅱ-L and Xho Ⅰ-B, C segment. The promoter region of polyhedrin gene of HcNPV genome DNA was sequenced. The sequences identified to the TATA box was found at the 5' flanking region of the polyhedrin gene approximately 21 bp upstream from the transcriptional start site. But CAAT-like box in the polyhedrin gene was not found in the sequences flanking the TATA-like box. Two fragments of tandem repeats with the sequence 5'-CTAATAT-3' and 5'-TAAATAA-3' were found between 83 and 50 or 25 upstream and 4 bp downstream from the translation start site. About 83 bp region upstream from the translational start site was highly AT(78%) rich. pUC8 plasmid vector and EcoR Ⅰ-H fragment were digested with BamH Ⅰ/EcoR Ⅰ and ligated to be named as pBE4. Bovine growth hormone gene(1.1kb) was inserted into BamH Ⅰ and Hind Ⅲ site of the pBE4 and named as pbGHL1. For the construction of recombinant viral DNA, pbGHL1 plasmid DNA and HcNPV DNA were cotrasfected S. frugiperda cell and selected polyhedra negative plaque, which was named as pBHcL1. Bovine growth hormone production was measured by radioimmunioassay method. The amount of bovine growth hormone produced by pbGHL1 was 0.09ng/ml and 0.07ng/ml in pbHcL1 respectively.