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使用天然聚丙烯酰胺凝胶电泳测定法对降钙素基因相关肽和肾上腺髓质素受体与 G 蛋白偶联的生化特性进行分析。

Biochemical characterization of G protein coupling to calcitonin gene-related peptide and adrenomedullin receptors using a native PAGE assay.

机构信息

Department of Biochemistry and Molecular Biology, University of Oklahoma Health Sciences Center, Oklahoma City, Oklahoma, USA.

Department of Biochemistry and Molecular Biology, University of Oklahoma Health Sciences Center, Oklahoma City, Oklahoma, USA

出版信息

J Biol Chem. 2020 Jul 10;295(28):9736-9751. doi: 10.1074/jbc.RA120.013854. Epub 2020 Jun 2.

Abstract

Calcitonin gene-related peptide (CGRP), adrenomedullin (AM), and adrenomedullin 2/intermedin (AM2/IMD) have overlapping and unique functions in the nervous and circulatory systems including vasodilation, cardioprotection, and pain transmission. Their actions are mediated by the class B calcitonin-like G protein-coupled receptor (CLR), which heterodimerizes with three receptor activity-modifying proteins (RAMP1-3) that determine its peptide ligand selectivity. How the three agonists and RAMPs modulate CLR binding to transducer proteins remains poorly understood. Here, we biochemically characterized agonist-promoted G protein coupling to each CLR·RAMP complex. We adapted a native PAGE method to assess the formation and thermostabilities of detergent-solubilized fluorescent protein-tagged CLR·RAMP complexes expressed in mammalian cells. Addition of agonist and the purified G protein surrogate mini-G (mG) yielded a mobility-shifted agonist·CLR·RAMP·mG quaternary complex gel band that was sensitive to antagonists. Measuring the apparent affinities of the agonists for the mG-coupled receptors and of mG for the agonist-occupied receptors revealed that both ligand and RAMP control mG coupling and defined how agonist engagement of the CLR extracellular and transmembrane domains affects transducer recruitment. Using mini-G and -G chimeras, we observed a coupling rank order of mG > mG > mG for each receptor. Last, we demonstrated the physiological relevance of the native gel assays by showing that they can predict the cAMP-signaling potencies of AM and AM2/IMD chimeras. These results highlight the power of the native PAGE assay for membrane protein biochemistry and provide a biochemical foundation for understanding the molecular basis of shared and distinct signaling properties of CGRP, AM, and AM2/IMD.

摘要

降钙素基因相关肽 (CGRP)、肾上腺髓质素 (AM) 和肾上腺髓质素 2/中介素 (AM2/IMD) 在神经系统和循环系统中具有重叠和独特的功能,包括血管舒张、心脏保护和疼痛传递。它们的作用是由 B 类降钙素样 G 蛋白偶联受体 (CLR) 介导的,该受体与三种受体活性修饰蛋白 (RAMP1-3) 异二聚化,决定其肽配体选择性。三种激动剂和 RAMP 如何调节 CLR 与转导蛋白的结合仍知之甚少。在这里,我们从生化角度表征了激动剂促进的 G 蛋白与每个 CLR·RAMP 复合物的偶联。我们改编了一种天然 PAGE 方法来评估在哺乳动物细胞中表达的荧光蛋白标记的 CLR·RAMP 复合物的形成和热稳定性。激动剂和纯化的 G 蛋白替代物 mini-G (mG) 的添加产生了一个迁移率发生变化的激动剂·CLR·RAMP·mG 四元复合物凝胶带,该带对拮抗剂敏感。测量激动剂与 mG 偶联受体的表观亲和力以及 mG 与激动剂占据的受体的亲和力表明,配体和 RAMP 都控制 mG 偶联,并且定义了激动剂与 CLR 细胞外和跨膜结构域的结合如何影响转导子的募集。使用 mini-G 和 -G 嵌合体,我们观察到每个受体的 mG > mG > mG 偶联等级。最后,我们通过表明它们可以预测 AM 和 AM2/IMD 嵌合体的 cAMP 信号强度,证明了天然凝胶测定的生理相关性。这些结果突出了天然 PAGE 测定在膜蛋白生物化学中的强大功能,并为理解 CGRP、AM 和 AM2/IMD 的共享和独特信号特性的分子基础提供了生化基础。

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