1986 Volume 99 Issue 4 Pages 1227-1236
A cytochrome b560-d complex, a terminal oxidase in the respiratory chain of Photobacterium phosphoreum grown under aerobic conditions, was purified to near homo-geneity. The purified oxidase complex is composed of equimolar amounts of two polypeptides with molecular weights of 41, 000 and 54, 000, as determined by gel electrophoresis in the presence of sodium dodecyl sulfate. It contains 10.2 nmol of protoheme and 22.5 nmol of iron/mg of protein.
The enzyme is a “cytochrome bd-type oxidase, ” showing absorption peaks at 560 and 625nm in its reduced minus oxidized difference spectrum at 77K. This oxidase combined with CO, and its CO difference spectrum at room temperature in the Soret region showed a peak at 418nm and a trough at 434nm. In addition, a trough at 560nm (cytochrome b), and a trough at 620nm and a peak at 639nm (cytochrome d) were observed in the CO-binding spectrum.
This cytochrome b560-d complex catalyzed the oxidation of tibiquino1-1 and ascorbate in the presence of N, N, N', N'-tetramethyl-p-phenylenediamine dihydrochloride or phenazine methosulfate. The oxidase activity required phospholipids and was inhibited by the respiratory inhibitors, KCN and NaN3, and the divalent cation, ZnSO4.
Formation of a membrane potential by the cytochrome b560-d complex reconstituted into liposomes was observed with the fluorescent dye, 3, 3'-dipropylthiodi-carbocyanine iodide, on the addition of ubiquinol-1, showing that the enzyme provided a coupling site for oxidative phosphorylation.