Identification of human CD93 as the phagocytic C1q receptor (C1qRp) by expression cloning

Author:

Steinberger Peter1,Szekeres Andreas2,Wille Stefan1,Stöckl Johannes1,Selenko Nicole1,Prager Elisabeth2,Staffler Günther2,Madic Otto1,Stockinger Hannes2,Knapp Walter12

Affiliation:

1. Institute of Immunology, University of Vienna , A-1090 Vienna, Austria

2. Institute of Immunology— Vienna International Research Cooperation Center at NFI, University of Vienna , A-1235 Vienna, Austria

Abstract

Abstract CD93 is a ∼120 kDa O-sialoglycoprotein that within the hematopoietic system is selectively expressed on cells of the myeloid lineage. So far, its primary structure and function were unknown. We used retroviral-expression cloning to isolate the CD93 cDNA. Sequence analysis revealed that CD93 is identical to a protein on human phagocytes termed C1q receptor (C1qRp). C1qRp was shown previously to mediate enhancement of phagocytosis in monocytes and was suggested to be a receptor of C1q and two other structurally related molecules. When studying CD93 transductants and control cells, we found that cells expressing CD93 have enhanced capacity to bind C1q. Furthermore, we show that immature dendritic cells (DC) express CD93/C1qRp, and mature DC, known to have reduced capacity for antigen uptake and to have lost the ability to phagocytose, show weak-to-negative CD93/C1qRp expression.

Funder

Austrian Science Fund

Competence Center “Bio-Molecular Therapeutics

Publisher

Oxford University Press (OUP)

Subject

Cell Biology,Immunology,Immunology and Allergy

Reference39 articles.

1. cDNA cloning and primary structure analysis of C1qR(P), the human C1q/MBL/SPA receptor that mediates enhanced phagocytosis in vitro;Nepomuceno;Immunity,1997

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