SHEDDING AND ISOLATION OF THE DELTA(6)-DESATURASE SYSTEM FROM RAT-LIVER MICROSOMES BY APPLICATION OF HIGH HYDROSTATIC-PRESSURE

A procedure using high hydrostatic pressure without detergent has been applied in this study to subfractionate the components of the Delta(6 )-desaturase system from the rat liver endoplasmic reticulum. Microsom es were suspended in a buffer containing liposomes made of phosphatidy lcholine. The mixture was placed in a sealed pressure bomb and subject ed to hydrostatic pressure of up to 1500 bars. Under these conditions the total desaturase activity was found in the liposomal fraction thus indicating that the three components of the desaturase system, namely NADH-cytochrome b(5) reductase, cytochrome b(5) and the Delta(6)-desa turase co-extracted. Size chromatography and FPLC of the released prot eins followed by SDS-PAGE confirmed the independent release of the thr ee components corresponding to the Delta(6)-desaturase system, Delta(6 )-Desaturase activity could be fully regenerated by mixing the aqueous dispersions of the three components without further purification. Our results indicate that these components are physically facing a simila r lipid environment in the microsomal membrane.