Ting Zhang, Ning Ma, Jiaxing Wang, Xiaoyun Min, Linlin Wei, Ke Li
{"title":"C5aR2 缺乏会减少 C5aR1 在中性粒细胞和巨噬细胞中的分布和表达。","authors":"Ting Zhang, Ning Ma, Jiaxing Wang, Xiaoyun Min, Linlin Wei, Ke Li","doi":"10.1155/2024/2899154","DOIUrl":null,"url":null,"abstract":"<p><p>As another receptor for complement activation product C5a, C5aR2 has been paid much attention these years. Although controversial and complex, its specific signals or roles in modulating the classic receptor C5aR1 have been investigated and gradually revealed. The hypothesis of the heterodimer of C5aR1 and C5aR2 has also been suggested and observed under extremely high C5a concentrations. In this article, we tried to investigate whether C5aR2 would affect C5aR1 expression under normal or inflammatory conditions in WT and <i>C5ar2</i> <sup><i>-/</i>-</sup> mice of C57BL/6 background. We focused on the innate immune cells-neutrophils and macrophages. The mRNA levels of <i>C5ar1</i> in normal kidney, liver, and the mRNA or protein levels of naïve-bone marrow and peripheral blood leukocytes and peritoneal M<i>φ</i>s were comparable between WT and <i>C5ar2</i> <sup><i>-/</i>-</sup> mice, indicating the technique of C5aR2 knockout did not affect the transcription of its neighboring gene C5aR1. However, the mean fluorescence intensity of surface C5aR1 on naïve circulating <i>C5ar2</i> <sup><i>-/</i>-</sup> neutrophils detected by FACS was reduced, which might be due to the reduced internalization of C5aR1 on <i>C5ar2</i> <sup><i>-/</i>-</sup> neutrophils. In the peritonitis model induced by <i>i.p</i>. injection of thioglycollate, more neutrophils were raised after 10 hr in <i>C5ar2</i> <sup><i>-/</i>-</sup> peritoneal cavity, indicating the antagonism of C5aR2 on C5aR1 signal in neutrophil chemotaxis. After 3 days of thioglycollate injection, the mainly infiltrating macrophages were comparable between WT and <i>C5ar2</i> <sup><i>-/</i>-</sup> mice, but the <i>C5ar1</i> mRNA and surface or total C5aR1 protein expression were both reduced in <i>C5ar2</i> <sup><i>-/</i>-</sup> macrophages, combined with our previous study of reduced chemokines and cytokines expression in <i>C5ar2</i> <sup><i>-/</i>-</sup> peritoneal macrophages, indicating that C5aR2 in macrophages may cooperate with C5aR1 inflammatory signals. Our article found C5aR2 deficiency lessened C5aR1 distribution and expression in neutrophils and macrophages with different functions, indicating C5aR2 might function differently in different cells.</p>","PeriodicalId":15952,"journal":{"name":"Journal of Immunology Research","volume":null,"pages":null},"PeriodicalIF":3.5000,"publicationDate":"2024-07-10","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://www.ncbi.nlm.nih.gov/pmc/articles/PMC11254461/pdf/","citationCount":"0","resultStr":"{\"title\":\"C5aR2 Deficiency Lessens C5aR1 Distribution and Expression in Neutrophils and Macrophages.\",\"authors\":\"Ting Zhang, Ning Ma, Jiaxing Wang, Xiaoyun Min, Linlin Wei, Ke Li\",\"doi\":\"10.1155/2024/2899154\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<p><p>As another receptor for complement activation product C5a, C5aR2 has been paid much attention these years. Although controversial and complex, its specific signals or roles in modulating the classic receptor C5aR1 have been investigated and gradually revealed. The hypothesis of the heterodimer of C5aR1 and C5aR2 has also been suggested and observed under extremely high C5a concentrations. In this article, we tried to investigate whether C5aR2 would affect C5aR1 expression under normal or inflammatory conditions in WT and <i>C5ar2</i> <sup><i>-/</i>-</sup> mice of C57BL/6 background. We focused on the innate immune cells-neutrophils and macrophages. The mRNA levels of <i>C5ar1</i> in normal kidney, liver, and the mRNA or protein levels of naïve-bone marrow and peripheral blood leukocytes and peritoneal M<i>φ</i>s were comparable between WT and <i>C5ar2</i> <sup><i>-/</i>-</sup> mice, indicating the technique of C5aR2 knockout did not affect the transcription of its neighboring gene C5aR1. However, the mean fluorescence intensity of surface C5aR1 on naïve circulating <i>C5ar2</i> <sup><i>-/</i>-</sup> neutrophils detected by FACS was reduced, which might be due to the reduced internalization of C5aR1 on <i>C5ar2</i> <sup><i>-/</i>-</sup> neutrophils. In the peritonitis model induced by <i>i.p</i>. injection of thioglycollate, more neutrophils were raised after 10 hr in <i>C5ar2</i> <sup><i>-/</i>-</sup> peritoneal cavity, indicating the antagonism of C5aR2 on C5aR1 signal in neutrophil chemotaxis. After 3 days of thioglycollate injection, the mainly infiltrating macrophages were comparable between WT and <i>C5ar2</i> <sup><i>-/</i>-</sup> mice, but the <i>C5ar1</i> mRNA and surface or total C5aR1 protein expression were both reduced in <i>C5ar2</i> <sup><i>-/</i>-</sup> macrophages, combined with our previous study of reduced chemokines and cytokines expression in <i>C5ar2</i> <sup><i>-/</i>-</sup> peritoneal macrophages, indicating that C5aR2 in macrophages may cooperate with C5aR1 inflammatory signals. 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C5aR2 Deficiency Lessens C5aR1 Distribution and Expression in Neutrophils and Macrophages.
As another receptor for complement activation product C5a, C5aR2 has been paid much attention these years. Although controversial and complex, its specific signals or roles in modulating the classic receptor C5aR1 have been investigated and gradually revealed. The hypothesis of the heterodimer of C5aR1 and C5aR2 has also been suggested and observed under extremely high C5a concentrations. In this article, we tried to investigate whether C5aR2 would affect C5aR1 expression under normal or inflammatory conditions in WT and C5ar2-/- mice of C57BL/6 background. We focused on the innate immune cells-neutrophils and macrophages. The mRNA levels of C5ar1 in normal kidney, liver, and the mRNA or protein levels of naïve-bone marrow and peripheral blood leukocytes and peritoneal Mφs were comparable between WT and C5ar2-/- mice, indicating the technique of C5aR2 knockout did not affect the transcription of its neighboring gene C5aR1. However, the mean fluorescence intensity of surface C5aR1 on naïve circulating C5ar2-/- neutrophils detected by FACS was reduced, which might be due to the reduced internalization of C5aR1 on C5ar2-/- neutrophils. In the peritonitis model induced by i.p. injection of thioglycollate, more neutrophils were raised after 10 hr in C5ar2-/- peritoneal cavity, indicating the antagonism of C5aR2 on C5aR1 signal in neutrophil chemotaxis. After 3 days of thioglycollate injection, the mainly infiltrating macrophages were comparable between WT and C5ar2-/- mice, but the C5ar1 mRNA and surface or total C5aR1 protein expression were both reduced in C5ar2-/- macrophages, combined with our previous study of reduced chemokines and cytokines expression in C5ar2-/- peritoneal macrophages, indicating that C5aR2 in macrophages may cooperate with C5aR1 inflammatory signals. Our article found C5aR2 deficiency lessened C5aR1 distribution and expression in neutrophils and macrophages with different functions, indicating C5aR2 might function differently in different cells.
期刊介绍:
Journal of Immunology Research is a peer-reviewed, Open Access journal that provides a platform for scientists and clinicians working in different areas of immunology and therapy. The journal publishes research articles, review articles, as well as clinical studies related to classical immunology, molecular immunology, clinical immunology, cancer immunology, transplantation immunology, immune pathology, immunodeficiency, autoimmune diseases, immune disorders, and immunotherapy.
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