Cytochemistry and reactive oxygen species: a retrospective

This retrospective reviews the methodology we have developed over several decades for detecting reactive oxygen species (ROS), using the activated polymorphonuclear leukocyte (PMN) as the paradigm of a cell which vigorously generates ROS through activation of NADPH oxidase. In the seventies, the sites of ROS generation by PMN were not clear from biochemical data, and we sought to develop new methods for the cytochemical localization of O^·– ₂, H₂O₂, and the H₂O₂-myeloperoxidase (MPO)-halide system. The H₂O₂-MPO-halide system in phagocytosing cells was localized at the fine structural level by our development of 3,3-diaminobenzidine (DAB) as a cytochemical probe for detecting peroxidase activities. Using DAB and exogenous H₂O₂, we confirmed that azurophil granules discharged MPO into the phagosome, and using particles coated with DAB and relying on endogenous H₂O₂ to yield oxidized DAB, H₂O₂ was localized to phagolysosomes. The subcellular sites of H₂O₂ generation were shown using cerium ions which react with H₂O₂ and precipitate electron opaque cerium perhydroxides (Ce(OH)₂OOH and Ce(OH)₃OOH). The results suggested that NADPH oxidase is associated with the plasmalemma, and that the enzyme enters the phagosome along with the invaginating plasmalemma, accounting for the presence of H₂O₂ in the phagosome. As O^·– ₂ is the major product of NADPH oxidase, its detection was of some importance. Based on the concept that O^·– ₂ oxidizes Mn²⁺ to Mn³⁺, and Mn³⁺ oxidizes DAB, a medium containing DAB-Mn²⁺ was used to localize sites of O^·– ₂ production in stimulated PMN. The localizations were, as expected, similar to those for H₂O₂. These techniques have been of considerable usefulness and in general provide the foundation for cytochemistry of ROS in other systems.Presented at the 36th Symposium of the Society for Histochemistry, 22 September 1994, Heidelberg, Germany