过敏毒素受体报告小鼠中过敏毒素受体表达及C3a/C5a功能的表征

Q2 Immunology and Microbiology Current Protocols in Immunology Pub Date : 2020-07-25 DOI:10.1002/cpim.100
Yves Laumonnier, Christian M. Karsten, Gabriele Köhl, Jörg Köhl
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引用次数: 5

摘要

过敏毒素(AT) C3a和C5a是C3和C5的效应分子,通过结合和激活其同源G蛋白偶联受体发挥多种生物学功能。C3a与C3a受体(C3aR)相互作用,而C5a及其初级降解产物C5a- desarg与C5aR1和C5aR2相互作用。在过去,对AT表达的分析一直受到旨在识别不同AT受体的抗体交叉反应的阻碍。此外,评估细胞特异性激活介导的效应一直很困难。在这里,floxed AT受体报告小鼠被描述为监测AT受体在细胞和组织中的表达的工具,并通过细胞特异性删除其同源AT受体来研究C3a和C5a的功能。©2020作者。基本方案1:floxed GFP-C5aR1敲入小鼠的基因分型支持方案1:lysmcree -C5aR1 -/-小鼠的基因分型基本方案2:floxed td番茄-C3aR和- td番茄-C5aR2敲入小鼠的基因分型支持方案2:基因组dna的制备基本方案3:使用floxed AT受体报告小鼠测定C5aR1、C5aR2和C3aR的表达支持方案3:使用C3aR特异性抗体测定C3aR的表达支持方案4:测定絮凝GFP-C5aR1、絮凝td番茄-C5aR2或- td番茄C3aR阳性细胞中C5aR1、C5aR2和C3aR mRNA表达基本方案4:分析GFP-C5aR1+细胞中C5aR1驱动的ERK1/2磷酸化基本方案5:评估絮凝td番茄-C3aR敲入小鼠获得的细胞中的C3aR功能-测定C3aR内化备选方案:c3a诱导细胞内Ca2+增加基本方案6:c5ar2驱动NK细胞产生IFN-γ支持方案5:用流式细胞术分离脾脏NK细胞
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Characterization of Anaphylatoxin Receptor Expression and C3a/C5a Functions in Anaphylatoxin Receptor Reporter Mice

The anaphylatoxins (AT) C3a and C5a are effector molecules of C3 and C5 exerting multiple biologic functions through binding and activation of their cognate G protein−coupled receptors. C3a interacts with the C3a receptor (C3aR), whereas C5a and its primary degradation product C5a-desArg engage C5aR1 and C5aR2. In the past, analysis of AT expression has been hampered by cross reaction of antibodies designed to recognize the different AT receptors. Furthermore, assessment of effects mediated by cell-specific activation has been difficult. Here, floxed AT receptor reporter mice are described as tools to monitor AT receptor expression in cells and tissues and to study the functions of C3a and C5a by cell-specific deletion of their cognate AT receptors. © 2020 The Authors.

Basic Protocol 1: Genotyping of floxed GFP-C5aR1 knockin mice

Support Protocol 1: Genotyping of LysMcre-C5ar1-/- mice

Basic Protocol 2: Genotyping of floxed tdTomato-C3aR and -tdTomato-C5aR2 knockin mice

Support Protocol 2: Preparation of genomic DNA

Basic Protocol 3: Determination of C5aR1, C5aR2, and C3aR expression using floxed AT receptor reporter mice

Support Protocol 3: Determination of C3aR expression using a C3aR-specific antibody

Support Protocol 4: Determination of C5aR1, C5aR2, and C3aR mRNA expression in floxed GFP-C5aR1, floxed tdTomato-C5aR2 or -tdTomato C3aR positive cells

Basic Protocol 4: Analysis of C5aR1-driven ERK1/2 phosphorylation in GFP-C5aR1+ cells

Basic Protocol 5: Assessment of C3aR functions in cells obtained from floxed tdTomato-C3aR knockin mice- Determination of C3aR internalization

Alternate Protocol: C3a-induced increase in intracellular Ca2+

Basic Protocol 6: C5aR2-driven IFN-γ production from NK cells

Support Protocol 5: Isolation of splenic NK cells by FACS

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Current Protocols in Immunology
Current Protocols in Immunology Immunology and Microbiology-Immunology
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