Localized apelin-17 analogue-bicelle interactions as a facilitator of membrane-catalyzed receptor recognition and binding

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS ACS Applied Bio Materials Pub Date : 2024-01-24 DOI:10.1016/j.bbamem.2024.184289
Trần Thanh Tâm Phạm , Alexandre Murza , Éric Marsault , John P. Frampton , Jan K. Rainey
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Abstract

The apelinergic system encompasses two peptide ligand families, apelin and apela, along with the apelin receptor (AR or APJ), a class A G-protein-coupled receptor. This system has diverse physiological effects, including modulating heart contraction, vasodilation/constriction, glucose regulation, and vascular development, with involvement in a variety of pathological conditions. Apelin peptides have been previously shown to interact with and become structured upon binding to anionic micelles, consistent with a membrane-catalyzed mechanism of ligand-receptor binding. To overcome the challenges of observing nuclear magnetic resonance (NMR) spectroscopy signals of a dilute peptide in biological environments, 19F NMR spectroscopy, including diffusion ordered spectroscopy (DOSY) and saturation transfer difference (STD) experiments, was used herein to explore the membrane-interactive behaviour of apelin. NMR-optimized apelin-17 analogues with 4-trifluoromethyl-phenylalanine at various positions were designed and tested for bioactivity through ERK activation in stably-AR transfected HEK 293 T cells. Far-UV circular dichroism (CD) spectropolarimetry and 19F NMR spectroscopy were used to compare the membrane interactions of these analogues with unlabelled apelin-17 in both zwitterionic/neutral and net-negative bicelle conditions. Each analogue binds to bicelles with relatively weak affinity (i.e., in fast exchange on the NMR timescale), with preferential interactions observed at the cationic residue-rich N-terminal and mid-length regions of the peptide leaving the C-terminal end unencumbered for receptor recognition, enabling a membrane-anchored fly-casting mechanism of peptide search for the receptor. In all, this study provides further insight into the membrane-interactive behaviour of an important bioactive peptide, demonstrating interactions and biophysical behaviour that cannot be neglected in therapeutic design.

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定位的芹菜素-17 类似物-双胞相互作用是膜催化受体识别和结合的促进因素
凋亡素能系统包括两个肽配体家族:凋亡素(apelin)和凋亡素(apela),以及凋亡素受体(AR 或 APJ)--一种 A 类 G 蛋白偶联受体。该系统具有多种生理效应,包括调节心脏收缩、血管扩张/收缩、血糖调节和血管发育,并涉及多种病理状况。以前的研究表明,凋亡肽与阴离子胶束结合后会发生相互作用并形成结构,这与配体-受体结合的膜催化机制一致。为了克服在生物环境中观察稀释肽的核磁共振(NMR)光谱信号所面临的挑战,本文使用 19F NMR 光谱,包括扩散有序光谱(DOSY)和饱和转移差(STD)实验,来探索芹菜素的膜相互作用行为。我们设计了在不同位置上含有 4-三氟甲基苯丙氨酸的 NMR 优化芹菜苷-17 类似物,并通过在稳定AR 转染的 HEK 293 T 细胞中激活 ERK 对其生物活性进行了测试。使用远紫外圆二色性(CD)分光测极法和 19F NMR 光谱法比较了这些类似物与未标记的 apelin-17 在齐聚物/中性和净阴性双细胞条件下的膜相互作用。每种类似物都以相对较弱的亲和力与双细胞结合(即在核磁共振时间尺度上快速交换),在多肽富含阳离子残基的 N 端和中长区域观察到优先的相互作用,而 C 端则没有受体识别的束缚,从而实现了多肽寻找受体的膜锚定蝇投机制。总之,这项研究进一步揭示了一种重要生物活性肽的膜相互作用行为,展示了治疗设计中不可忽视的相互作用和生物物理行为。
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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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