Intravenous immunoglobulin skews macrophages to an anti-inflammatory, IL-10-producing activation state

被引:36
|
作者
Kozicky, Lisa K. [1 ]
Zhao, Zheng Yu [1 ]
Menzies, Susan C. [1 ]
Fidanza, Mario [2 ,3 ]
Reid, Gregor S. D. [2 ,3 ]
Wilhelmsen, Kevin [4 ]
Hellman, Judith [4 ]
Hotte, Naomi [5 ]
Madsen, Karen L. [5 ]
Sly, Laura M. [1 ]
机构
[1] British Columbia Childrens Hosp, Child & Family Res Inst, Michael Cuccione Childhood Canc Res Program, Div Gastroenterol,Dept Pediat, Vancouver, BC V6H 3V4, Canada
[2] British Columbia Childrens Hosp, Child & Family Res Inst,Dept Pediat, Michael Cuccione Childhood Canc Res Program, Div Oncol Hematol & Blood & Marrow Transplantat, Vancouver, BC V6H 3V4, Canada
[3] Univ British Columbia, Vancouver, BC V5Z 1M9, Canada
[4] Univ Calif San Francisco, Dept Anesthesia & Perioperat Care, San Francisco, CA 94143 USA
[5] Univ Alberta, Dept Med, Div Gastroenterol, Edmonton, AB, Canada
关键词
macrophage activation; regulatory macrophages; Fc receptors; map kinases; sepsis; HUMAN REGULATORY MACROPHAGES; CYTOKINE PRODUCTION; ALTERNATIVE ACTIVATION; IL-10; MECHANISMS; EXPRESSION; RESPONSES; LIGATION; KINASE; MOUSE;
D O I
10.1189/jlb.3VMA0315-078R
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Intravenous Ig is used to treat autoimmune or autoinflammatory disorders, but themechanism by which it exerts its immunosuppressive activity is not understood completely. To examine the impact of intravenous Ig on macrophages, we compared cytokine production by LPS-activated macrophages in the presence and absence of intravenous Ig. Intravenous Ig treatment induced robust production of IL-10 in response to LPS, relative to LPS stimulation alone, and reduced production of proinflammatory cytokines. This anti-inflammatory, intravenous Ig-induced activation was sustained for 24 h but could only be induced if intravenous Ig were provided within 1 h of LPS stimulation. Intravenous Ig activation led to enhanced and prolonged activation of MAPKs, Erk1/2, p38, and Erk5, and inhibition of each reduced intravenous Ig-induced IL-10 production and suppression of IL-12/23p40. IL-10 production occurred rapidly in response to intravenous Ig + LPS and was sufficient to reduce proinflammatory IL-12/23p40 production in response to LPS. IL-10 induction and reduced IL-12/23p40 production were transcriptionally regulated. IL-10 played a direct role in reducing proinflammatory cytokine production by macrophages treated with intravenous Ig + LPS, as macrophages from mice deficient in the IL-10R beta chain or in IL-10 were compromised in their ability to reduce proinflammatory cytokine production. Finally, intraperitoneal injection of intravenous Ig or intravenous Ig + LPS into mice activated macrophages to produce high levels of IL-10 during subsequent or concurrent LPS challenge, respectively. These findings identify IL-10 as a key anti-inflammatory mediator produced by intravenous Ig-treated macrophages and provide insight into a novel mechanism by which intravenous Ig may dampen down inflammatory responses in patients with autoimmune or autoinflammatory diseases.
引用
收藏
页码:983 / 994
页数:12
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