Inflammation-induced proteolytic processing of the SIRPα cytoplasmic ITIM in neutrophils propagates a proinflammatory state

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作者
Ke Zen
Yalan Guo
Zhen Bian
Zhiyuan Lv
Dihan Zhu
Hiroshi Ohnishi
Takashi Matozaki
Yuan Liu
机构
[1] Jiangsu Engineering Research Center for MicroRNA Biology and Biotechnology,Department of Biology
[2] State Key Laboratory of Pharmaceutical Biotechnology,undefined
[3] Nanjing University School of Life Sciences,undefined
[4] Center for Inflammation,undefined
[5] Immunity and Infection,undefined
[6] Georgia State University,undefined
[7] PO Box 4010,undefined
[8] Atlanta,undefined
[9] Georgia 30303,undefined
[10] USA,undefined
[11] Laboratory of Biosignal Sciences,undefined
[12] Institute for Molecular and Cellular Regulation,undefined
[13] Gunma University,undefined
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Signal regulatory protein α (SIRPα), an immunoreceptor tyrosine-based inhibitory motif (ITIM)-containing receptor, is an essential negative regulator of leukocyte inflammatory responses. Here we report that SIRPα cytoplasmic signalling ITIMs in neutrophils are cleaved during active inflammation and that the loss of SIRPα ITIMs enhances the polymorphonuclear leukocyte (PMN) inflammatory response. Using human leukocytes and two inflammatory models in mice, we show that the cleavage of SIRPα ITIMs in PMNs but not monocytes occurs at the post-acute stage of inflammation and correlates with increased PMN recruitment to inflammatory loci. Enhanced transmigration of PMNs and PMN-associated tissue damage are confirmed in mutant mice expressing SIRPα but lacking the ITIMs. Moreover, the loss of SIRPα ITIMs in PMNs during colitis is blocked by an anti-interleukin-17 (IL-17) antibody. These results demonstrate a SIRPα-based mechanism that dynamically regulates PMN inflammatory responses by generating a CD47-binding but non-signalling SIRPα ‘decoy’.
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