Independent Mechanisms for Macrophage Binding and Macrophage Phagocytosis of Damaged Erythrocytes : Evidence of Receptor Cooperativity

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Arteriosclerosis, Thrombosis, and Vascular Biology. 1997;17:3442-3448

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(Arteriosclerosis, Thrombosis, and Vascular Biology. 1997;17:3442-3448.)
© 1997 American Heart Association, Inc.

Articles

Independent Mechanisms for Macrophage Binding and Macrophage Phagocytosis of Damaged Erythrocytes

Evidence of Receptor Cooperativity

Gilberto R. Sambrano; Valeska Terpstra; ; Daniel Steinberg

From the Department of Medicine, University of California San Diego, La Jolla, Calif.

Abstract The binding and phagocytosis of oxidatively damagedred blood cells (OxRBCs) by mouse peritoneal macrophages canbe inhibited by oxidatively modified LDL (OxLDL), implying somecommonality at their receptor-binding domains. Studies frommany different laboratories support the view that OxRBC bindingis due to the disruption of plasma membrane phospholipid asymmetryand the subsequent exposure of phosphatidylserine (PS) on theouter membrane leaflet. Presumably, oxidation of LDL createsa surface structure on it in some way homologous to the PS-richdomain on OxRBCs. Apoptotic cells in some instances are alsorecognized because of PS exposure on the outer leaflet of themembrane, and apoptotic cells are a common feature of atherosclerotic lesions.In the present studies, the mechanisms of binding and internalizationof cells recognized by virtue of their membrane PS were studiedusing OxRBCs or vanadate-treated erythrocytes (VaRBCs) as models.Disruption of phospholipid asymmetry with vanadate produced cellsthat were bound by macrophages in the same divalent cation–dependentmanner as OxRBCs. However, whereas OxRBCs were rapidly phagocytosed,VaRBCs were not. Stimulation of mouse macrophages with phorbolmyristate acetate resulted in a concentration-dependent inductionof phagocytosis of bound VaRBCs, an effect that could be preventedby the protein kinase C inhibitor staurosporine. Because phagocytosis ofOxRBCs occurred unassisted, we speculated that there must be additionalmembrane changes induced by oxidation (over and above the disruptionof phospholipid asymmetry) that contribute to phagocytosis ofOxRBCs, possibly resulting in the ligation of a distinct receptor thatdoes not necessarily contribute to adherence. This proposalis supported by the finding that ligation of macrophage Fc ${gamma}$ receptorsby the anti-Fc ${gamma}$ RII/RIII antibody 2.4G2 triggers the phagocytosisof bound VaRBCs. Phagocytosis is also triggered by subthresholdopsonization of VaRBC, ie, by antibody concentrations that donot by themselves cause binding and phagocytosis of native RBCs. Finally,treatment with low concentrations of glutaraldehyde, which causesmembrane protein cross-linking, promotes the phagocytosis ofVaRBCs, but, at the low concentration used, has little or noeffect on binding and phagocytosis of native RBCs. We suggestthat the internalization of damaged cells, bound because ofPS exposure, requires the cooperation of a PS-binding receptorwith at least one additional receptor to trigger an intracellularsignaling pathway to initiate phagocytosis.

Key Words: macrophages • apoptosis • scavenger receptors

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