Subcellular localization of human monocyte interleukin 1: evidence for an inactive precursor molecule and a possible mechanism for IL 1 release.
Open Access
- 15 June 1987
- journal article
- research article
- Published by Oxford University Press (OUP) in The Journal of Immunology
- Vol. 138 (12) , 4249-4255
- https://doi.org/10.4049/jimmunol.138.12.4249
Abstract
IL 1 activity, as assayed by the proliferation of responsive mouse thymocytes and a human astrocytoma cell line, was detected on the membrane of 1% paraformaldehyde-fixed activated human monocytes. Resting, unactivated monocytes did not display IL 1 activity. Maximum induction of membrane IL 1 was obtained from monocytes treated with polyclonal activators, such as LPS or Staphylococcus aureus, whereas adherence was a weak inducer of membrane IL 1. Isolated cell compartments as plasma membranes, crude lysosomes, and crude cytosol from activated human monocytes expressed significant IL 1 activity, whereas the endoplasmic reticulum showed no IL 1 activity. Exposure to trypsin of either fixed, activated human monocytes or cell compartments from unfixed monocytes, revealed biologically active IL 1 in the membrane, crude lysosome, and crude cytosol, but not in the endoplasmic reticulum. The IL 1 activity in the purified cytosol, prepared by extraction with digitonin, was considerably increased by the trypsin treatment, whereas the increase in IL 1 activity within crude lysosomes and plasma membranes was less. The cell compartments from nonactivated monocytes did not express active IL 1 and trypsin treatment revealed no active IL 1, suggesting the absence of a pool of the trypsin-sensitive form of IL 1. The data confirm the presence of membrane-bound IL 1 in activated human monocytes and indicate that an inactive precursor molecule can be found in the cytosol of such cells. Furthermore, the absence of IL 1 activity either in its active form or as the inactive precursor in the endoplasmic reticulum suggests that IL 1 is not a conventionally secreted protein. Because IL 1 was found in the cytosol as a precursor and in the lysosomal fractions in an active form, these data suggest that after the synthesis and processing of the cytosolic precursor, the 17-kda IL 1, is released via lysosomal vesicles.This publication has 21 references indexed in Scilit:
- Low and high affinity cellular receptors for interleukin 2. Implications for the level of Tac antigen.The Journal of Experimental Medicine, 1984
- Quantitation of intracellular membrane-bound enzymes and receptors in digitonin-permeabilized cellsAnalytical Biochemistry, 1983
- Tumoricidal activity of human monocytes activated in vitro by free and liposome-encapsulated human lymphokines.Journal of Clinical Investigation, 1983
- Acidification of macrophage and fibroblast endocytic vesicles in vitro.Proceedings of the National Academy of Sciences, 1983
- A simple and rapid method for the preparation of plasma membranesBiochimica et Biophysica Acta (BBA) - Biomembranes, 1983
- Relationship between production and release of lymphocyte-activating factor (interleukin 1) by murine macrophagesCellular Immunology, 1981
- An improved technique for the negative selection of large numbers of human lymphocytes and monocytes by counterflow centrifugation-elutriationCellular Immunology, 1980
- Membrane Association may Limit the Use of Acid Phosphatase as a Lysosomal MarkerBiochemical Society Transactions, 1978
- Synthesis and Secretion of a Mitogenic Protein by Macrophages: Description of a Superinduction PhenomenonThe Journal of Immunology, 1977
- Studies on Thiols. I. Oxidation of Thiol Groups by 2,6-Dichlorophenol Indophenol1Journal of the American Chemical Society, 1955