ENRICHMENT OF PENICILLIUM-CHRYSOGENUM MICROBODIES BY ISOPYCNIC CENTRIFUGATION IN NYCODENZ AS VISUALIZED WITH IMMUNOELECTRON MICROSCOPY

A procedure to enrich microbodies from Penicillium chrysogenum and a m ethod to evaluate the purity and integrity of the microbodies are desc ribed. As a P. chrysogenum microbody marker acyltransferase (AT) was u sed. The P, chrysogenum hyphae were converted into protoplasts with No vozym 234. In Percoll-sucrose buffer the protoplasts were separated fr om mycelial debris after 10 000 X g centrifugation. Purified protoplas ts were lysed, and the cell homogenate was centrifuged to form a 14 00 0 X g pellet. After 2 h, 45 000 X g isopycnic centrifugation of the 14 000 X g pellet on a continuous 20-60% nycodenz gradient, ten fraction s were collected. The fractions were analyzed for AT containing microb odies by immune-blotting and immune-electron microscopy. The results s howed that AT-microbodies are enriched in the 38% nycodenz fraction. T he microbodies had a diameter of 400 to 500 nm, revealed an intact sin gle membrane and confined AT. The estimated equilibrium density of the P. chrysogenum microbodies was 1.20 g ml(-1) as deduced from the 38% (w/v) nycodenz concentration.