Lysosomal Glycosidases in Mouse Peritoneal Macrophages Stimulated In Vitro With Soluble and Insoluble Glycans

Mouse peritoneal macrophages stimulated with insoluble glycans in vitro release high amounts of acid hydrolases, N‐acetyl‐ β ‐D‐glucosaminidase, β ‐D‐glucuronidase, and β ‐D‐galactosidase. The most potent of the stimulatory glycans is a β ‐1,3‐D‐glucan isolated from yeast cell walls. Up to 50% of total enzyme activity was found in the medium after stimulation with this glycan for three days. Agarose, another insoluble glycan containing an alternating sequence of the disaccharide β ‐1,3‐D‐galactose‐ α ‐1,4‐3,6‐anhydro‐L‐galactose units was less potent. The soluble β ‐1,3‐D‐glucan laminaran, which also contains small amounts of mannitol, was not able to induce release of acid glycosidases from macrophages. The release was independent of serum since macrophages cultured under serum‐free conditions showed nearly the same pattern of enzyme activities, both in the cells and media. There was no increased release of the acid hydrolase α ‐D‐mannosidase after stimulation with the insoluble β ‐1,3‐D‐glucan for three days. The release of the lysosomal glycosidases was not due to cell death, since only small amounts of the cytoplasmic enzyme lactate dehydrogenase were found in the culture media. Insoluble polystyrene latex particles were not able to stimulate mouse macrophages to release lysosomal glycosidases. Tritiated glycans (amylose, dextran, laminaran, the insoluble β ‐1,3‐D‐glucan, and agarose) and the p‐nitrophenyl‐glycopyranoside derivatives were used as substrates to investigate whether the macrophages contained or released glucanases capable of degrading α ‐1,4‐D‐glucans, α ‐1‐6‐D‐glucans, β ‐1,3‐D‐glucans, and agarose respectively. We conclude that the glycans were not degraded in macrophage cultures during the time period tested nor were the enzymes induced in macrophages by the glycans during in vitro culture for seven days.