4.7 Article

The acute-phase protein α1-acid glycoprotein (AGP) induces rises in cytosolic Ca2+ in neutrophil granulocytes via sialic acid binding immunoglobulin-like lectins (Siglecs)

Journal

FASEB JOURNAL
Volume 21, Issue 14, Pages 4059-4069

Publisher

WILEY
DOI: 10.1096/fj.07-8534com

Keywords

orosomucoid; plasma protein; calcium signaling; carbohydrate; L-selectin; phagocyte

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We studied whether the acute-phase protein alpha(1)-acid glycoprotein (AGP) induces rises in [Ca2+](i) in neutrophils and sought to identify the corresponding AGP receptor (or receptors). We found that AGP elicited a minimal rise in [Ca2+] i in Fura-2-loaded neutrophils, and this response was markedly enhanced by pretreatment with anti-L-selectin antibodies. (The EC50 value of the AGP-induced Ca2+ response was 9 mu g/ml.) Activation of phospholipase-C, Src tyrosine kinases, and PI3 kinases proved to be essential for the AGP-mediated increase in [Ca2+] i, whereas the p38 MAPK and SYK signaling pathways were not involved. Furthermore, antibodies against sialic acid binding, immunoglobulin-like lectin 5 (Siglec-5) and oligosaccharide 3 '- sialyl-lactose both antagonized the AGP-induced response and caused an immediate increase in [Ca2+] i in anti-L-selectin-treated neutrophils, which indicates a signaling capacity of Siglec-5. We used modified forms of AGP (treated with mild periodate or neuraminidase) to establish the importance of sialic acid residues. The modified forms of AGP caused a much smaller rise in [Ca2+] i than did unaltered AGP. Affinity chromatography confirmed that unchanged AGP, but not neuraminidase-treated AGP, bound to Siglec-5. Our report provides the first evidence for a signaling capacity by AGP through a defined receptor. Pre-engagement of L-selectin significantly enhanced this signaling capacity. -Gunnarsson, P., Levander, L., Pahlsson, P., Grenegard, M. The acute- phase protein alpha(1)- acid glycoprotein (AGP) induces rises in cytosolic Ca2+ in neutrophil granulocytes via sialic acid binding immunoglobulin- like lectins (Siglecs).

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