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Atlas of the anatomical localization of atypical chemokine receptors in healthy mice

CCL21型 生物 趋化因子受体 C-C趋化因子受体7型 趋化因子 20立方厘米 C-C趋化因子受体6型 CCL19型 CCR1 CCL25型 CCR10 细胞生物学 趋化因子受体 趋化因子受体CCR5 CXCL16型 CXCL2型 CCL5 CCL7型 免疫学 受体 T细胞 免疫系统 白细胞介素2受体 生物化学
作者
Serena Melgrati,Egle Radice,Rafet Ameti,Elin Hub,Sylvia Thelen,Paweł Pelczar,David Jarrossay,Antal Rot,Marcus Thelen
出处
期刊:PLOS Biology [Public Library of Science]
卷期号:21 (5): e3002111-e3002111 被引量:3
标识
DOI:10.1371/journal.pbio.3002111
摘要

Atypical chemokine receptors (ACKRs) scavenge chemokines and can contribute to gradient formation by binding, internalizing, and delivering chemokines for lysosomal degradation. ACKRs do not couple to G-proteins and fail to induce typical signaling induced by chemokine receptors. ACKR3, which binds and scavenges CXCL12 and CXCL11, is known to be expressed in vascular endothelium, where it has immediate access to circulating chemokines. ACKR4, which binds and scavenges CCL19, CCL20, CCL21, CCL22, and CCL25, has also been detected in lymphatic and blood vessels of secondary lymphoid organs, where it clears chemokines to facilitate cell migration. Recently, GPR182, a novel ACKR-like scavenger receptor, has been identified and partially deorphanized. Multiple studies point towards the potential coexpression of these 3 ACKRs, which all interact with homeostatic chemokines, in defined cellular microenvironments of several organs. However, an extensive map of ACKR3, ACKR4, and GPR182 expression in mice has been missing. In order to reliably detect ACKR expression and coexpression, in the absence of specific anti-ACKR antibodies, we generated fluorescent reporter mice, ACKR3GFP/+, ACKR4GFP/+, GPR182mCherry/+, and engineered fluorescently labeled ACKR-selective chimeric chemokines for in vivo uptake. Our study on young healthy mice revealed unique and common expression patterns of ACKRs in primary and secondary lymphoid organs, small intestine, colon, liver, and kidney. Furthermore, using chimeric chemokines, we were able to detect distinct zonal expression and activity of ACKR4 and GPR182 in the liver, which suggests their cooperative relationship. This study provides a broad comparative view and a solid stepping stone for future functional explorations of ACKRs based on the microanatomical localization and distinct and cooperative roles of these powerful chemokine scavengers.
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