Optimization of a PCR Method for Detection of Lipase Gene in Bacillus subtilis

Lipases catalyze hydrolysis and synthesis of triacylglycerols. these enzymes,especially the microbial ones, have wide commercial and industrial usage. bacillussubtilis lipase has interesting properties such as small size and tolerance to basic ph;therefore, developing techniques for its recognition and isolation is the focus ofresearch in many laboratories. in the present study, two factors i.e. mgcl2concentration and annealing temperature were manipulated for the optimization ofthe polymerase chain reaction (pcr) condition. as for the mgcl2 concentration, 2.5mm produced the best results when the annealing temperature was kept at 55 oc.regarding the annealing temperatures, the best amplification was obtained at 63.9oc. it can be concluded that the pcr conditions for the detection of lipase gene inbacillus subtilis has been optimized and can be used for the screening and isolationof these bacaterial strains.