In Vivo Depletion of CD206+ M2 Macrophages Exaggerates Lung Injury in Endotoxemic Mice

Although phenotypically polarized macrophages are now generally classified into two major subtypes termed proinflammatory M1 and anti-inflammatory M2 macrophages, a contributory role of lung M2 macrophages in the pathophysiological features of acute lung injury is not fully understood. Herein, we sh...

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Veröffentlicht in:	The American journal of pathology 2015, Vol.185 (1), p.162-171
Hauptverfasser:	Kambara, Kenta, Ohashi, Wakana, Tomita, Kengo, Takashina, Michinori, Fujisaka, Shiho, Hayashi, Ryuji, Mori, Hisashi, Tobe, Kazuyuki, Hattori, Yuichi
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Schlagworte:	Acute Lung Injury - metabolism Animals Bronchoalveolar Lavage Fluid Cell Membrane - metabolism Chromosomes, Artificial, Bacterial Endotoxemia - metabolism Endotoxemia - pathology Exons Humans Inflammation - pathology Lectins, C-Type - genetics Lectins, C-Type - metabolism Lipopolysaccharides Lung - metabolism Macrophages - cytology Macrophages - metabolism Mannose-Binding Lectins - genetics Mannose-Binding Lectins - metabolism Mice Mice, Inbred C57BL Mice, Transgenic Neutrophils - cytology NF-kappa B - metabolism Pathology Phenotype Rabbits Receptors, Cell Surface - genetics Receptors, Cell Surface - metabolism RNA, Messenger - metabolism Transcription Factor AP-1 - metabolism
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creator	Kambara, Kenta Ohashi, Wakana Tomita, Kengo Takashina, Michinori Fujisaka, Shiho Hayashi, Ryuji Mori, Hisashi Tobe, Kazuyuki Hattori, Yuichi
description	Although phenotypically polarized macrophages are now generally classified into two major subtypes termed proinflammatory M1 and anti-inflammatory M2 macrophages, a contributory role of lung M2 macrophages in the pathophysiological features of acute lung injury is not fully understood. Herein, we show in an endotoxemic murine model that M2 macrophages serve as key anti-inflammatory cells that play a regulatory role in the severity of lung injury. To study whether M2 macrophages can modify inflammation, we depleted M2 macrophages from lungs of CD206-diphtheria toxin (DT) receptor transgenic (Tg) mice during challenge with lipopolysaccharide. The i.p. administration of DT depleted CD206-positive cells in bronchoalveolar lavage fluid. The use of M2 macrophage markers Ym1 and arginase-1 identified pulmonary CD206-positive cells as M2 macrophages. A striking increase in neutrophils in bronchoalveolar lavage fluid cell contents was found in DT-treated CD206-DT receptor Tg mice. In CD206-DT receptor Tg mice given DT, endotoxin challenge exaggerated lung inflammation, including up-regulation of proinflammatory cytokines and increased histological lung damage, but the endotoxemia-induced increase in NF-κB activity was significantly reduced, suggesting that M2 phenotype-dependent counteraction of inflammatory insult cannot be attributed to the inhibition of the NF-κB pathway. Our results indicate a critical role of CD206-positive pulmonary macrophages in triggering inflammatory cascade during endotoxemic lung inflammation.
doi_str_mv	10.1016/j.ajpath.2014.09.005
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In CD206-DT receptor Tg mice given DT, endotoxin challenge exaggerated lung inflammation, including up-regulation of proinflammatory cytokines and increased histological lung damage, but the endotoxemia-induced increase in NF-κB activity was significantly reduced, suggesting that M2 phenotype-dependent counteraction of inflammatory insult cannot be attributed to the inhibition of the NF-κB pathway. 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In CD206-DT receptor Tg mice given DT, endotoxin challenge exaggerated lung inflammation, including up-regulation of proinflammatory cytokines and increased histological lung damage, but the endotoxemia-induced increase in NF-κB activity was significantly reduced, suggesting that M2 phenotype-dependent counteraction of inflammatory insult cannot be attributed to the inhibition of the NF-κB pathway. 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Herein, we show in an endotoxemic murine model that M2 macrophages serve as key anti-inflammatory cells that play a regulatory role in the severity of lung injury. To study whether M2 macrophages can modify inflammation, we depleted M2 macrophages from lungs of CD206-diphtheria toxin (DT) receptor transgenic (Tg) mice during challenge with lipopolysaccharide. The i.p. administration of DT depleted CD206-positive cells in bronchoalveolar lavage fluid. The use of M2 macrophage markers Ym1 and arginase-1 identified pulmonary CD206-positive cells as M2 macrophages. A striking increase in neutrophils in bronchoalveolar lavage fluid cell contents was found in DT-treated CD206-DT receptor Tg mice. 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subjects	Acute Lung Injury - metabolism Animals Bronchoalveolar Lavage Fluid Cell Membrane - metabolism Chromosomes, Artificial, Bacterial Endotoxemia - metabolism Endotoxemia - pathology Exons Humans Inflammation - pathology Lectins, C-Type - genetics Lectins, C-Type - metabolism Lipopolysaccharides Lung - metabolism Macrophages - cytology Macrophages - metabolism Mannose-Binding Lectins - genetics Mannose-Binding Lectins - metabolism Mice Mice, Inbred C57BL Mice, Transgenic Neutrophils - cytology NF-kappa B - metabolism Pathology Phenotype Rabbits Receptors, Cell Surface - genetics Receptors, Cell Surface - metabolism RNA, Messenger - metabolism Transcription Factor AP-1 - metabolism
title	In Vivo Depletion of CD206+ M2 Macrophages Exaggerates Lung Injury in Endotoxemic Mice
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