Protease from various sources have been studied biotecnologically. For biotechnological applications, one highly preferred enzyme is protease. There have been no reports of cloned genes encoding digestive proteases in the Laccotrephes japonenis, Ranatra unicolor, Muljarus japonicus. These insects are considered to be a predator of aquatic insects. RT-PCR was used to amplify cDNA fragments for digestive proteases from total RNA the hole body of the insects. The flanking sequences of the 5'- and 3'- end of the these genes were characterized by RACE-PCR. Sequence analysis showed that these genes contained complete ORF. The deduced amino acid sequences of these protease showed 62% identity to the serine protease of Creontiades dilutus, 58% to Lygus loneolaris trypsin-like serine proteinase, 54% to Triatonatoma infestans salivary trypsin. To generate Laccotrephes japonensis serine protease, the DNA fragment coding for serine protease is cloning into suttle vector pBACⅠ, named pBAC1-JG and infected to Spodoptera frugiperda (sf9) insect cell. The cDNA encoding JG was expressed as a 32-kDa polypeptide in baculovirus infected insect cells and the recombinant protein showed activity in the protease enzyme assay using gelatin as a substrate.

• Kwan-Ho Park(Department of Agricultural Biology, NAAS, RDA)
• Young-Cheol Choi(Department of Agricultural Biology, NAAS, RDA)
• Jong-Gil Kim(Department of Agricultural Biology, NAAS, RDA)
• Ji-Young Choi(Department of Agricultural Biology, NAAS, RDA)
• Won-Tae Kim(Department of Agricultural Biology, NAAS, RDA)
• Si-Kab Nho(College of Agriculture and Life sciences, Kyungpook National University)
• Jae-Sam Hwang(Department of Agricultural Biology, NAAS, RDA)