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Stimulus‐specific defect in the phagocytic pathways of annexin 1 null macrophages
Author(s) -
Yona Simon,
Buckingham Julia C,
Perretti Mauro,
Flower Roderick J
Publication year - 2004
Publication title -
british journal of pharmacology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.432
H-Index - 211
eISSN - 1476-5381
pISSN - 0007-1188
DOI - 10.1038/sj.bjp.0705858
Subject(s) - zymosan , phagocytosis , annexin , annexin a5 , macrophage , microbiology and biotechnology , biology , annexin a2 , annexin a1 , reactive oxygen species , chemistry , immunology , flow cytometry , biochemistry , in vitro
The role of the glucocorticoid‐regulated protein annexin 1 during the process of phagocytosis has been studied using annexin 1 null peritoneal macrophages. Wild type and annexin 1 null macrophages were incubated with several distinct phagocytic targets. No differences were observed in rate or the maximal response with respect to IgG complexes or opsonised zymosan phagocytosis, as assessed by monitoring the production of reactive oxygen species. When annexin 1 null macrophages were incubated with non‐opsonised zymosan particles, they exhibited impaired generation of reactive oxygen species, which was linked to a defect in binding of cells to the particles, as determined with fluorescent zymosan. This phenomenon was further confirmed by electron microscopy analysis, where annexin 1 null macrophages internalised fewer non‐opsonised zymosan particles. Specific alterations in macrophage plasma membrane markers were observed in the annexin 1 null cells. Whereas no differences in dectin‐1 and Fc γ R II/III expression were measured between the two genotypes, decreased membrane CD11b and F4/80 levels were measured selectively in macrophages lacking annexin 1. These cells also responded with an enhanced release of PGE 2 and COX‐2 protein expression following addition of the soluble stimulants, LPS and heat‐activated IgG. In conclusion, these results suggest that participation of endogenous annexin 1 during zymosan phagocytosis is critical and that this protein plays a tonic inhibitory role during macrophage activation.British Journal of Pharmacology (2004) 142 , 890–898. doi: 10.1038/sj.bjp.0705858

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