eng Oriental Scientific Publishing Company Biosciences Biotechnology Research Asia 0973-1245 2019-12-28 16 4 817 826 10.13005/bbra/2799 34870 article Endang Rahmawati 1 Abinawanto 1 Is Helianti 2 Department of Biology, Faculty of Mathematics and Natural Science, University of Indonesia, Depok, Jawa Barat, Indonesia Center for Bioindustrial Technology, Agency of Assessment and Application of Technology (BPPT), 611/614 Building, LAPTIAB-BPPT, PUSPITEK-Serpong, Tangerang Selatan 15314, Indonesia Proteases are potential enzymes that utilized in various industrial fields, and the demand of these enzymes is increasing. Bacillus halodurans CM1 is Indonesia indigenous bacterium which is detected to be able to produce alkalotermophilic protease enzyme. In this study, we subcloned the protease gene consist of Open Reading Frame of protease gene and its promoter from Bacillus halodurans CM1 in Bacillus subtilis DB104 via conjugation, and analyzed the expression of the recombinant protease. The protease gene is 1 417 bp length including the open reading frame and the promoter, and obtained by PCR and cloned into pGEM T easy. After confirmed by sequencing, the gene was subcloned into vector pBBRE194, then the recombinant plasmid was transformed into E. coli S17-1. This E.coli was then conjugated to Bacillus subtilis DB104. The target recombinant B. subtilis DB104 has been obtained confirmed by plasmid verification and erythromycin resistance. The recombinant protease produced showed the highest enzyme activity at 50^oC and pH 9 (with pH range 5-9) which with protease activity 13.66 U/mL. https://www.biotech-asia.org/vol16no4/subcloning-and-expression-of-a-protease-gene-from-bacillus-halodurans-cm1-in-bacillus-subtilis-db104/ Bacillus Halodurans CM1; Bacillus Subtlis DB104; Conjugation; Expression; Protease Gene; Subcloning