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人激肽B1受体在中国仓鼠卵巢细胞中的稳定表达。配体结合和效应途径的表征。

Stable expression of the human kinin B1 receptor in Chinese hamster ovary cells. Characterization of ligand binding and effector pathways.

作者信息

Austin C E, Faussner A, Robinson H E, Chakravarty S, Kyle D J, Bathon J M, Proud D

机构信息

Department of Medicine, Johns Hopkins University School of Medicine, Baltimore, Maryland 21224-6801, USA.

出版信息

J Biol Chem. 1997 Apr 25;272(17):11420-5. doi: 10.1074/jbc.272.17.11420.

DOI:10.1074/jbc.272.17.11420
PMID:9111052
Abstract

To delineate ligand binding and functional characteristics of the human B1 kinin receptor, a stable clone of Chinese hamster ovary cells expressing a single class of binding sites for [3H]des-Arg10-lysylbradykinin with a Kd of 0.3 nM and a Bmax of 38 fmol/mg protein ( approximately 40,000 receptors/cell) was isolated. Studies with peptide analogs showed that a lysine residue at position 1 (based on the lysylbradykinin sequence) of ligands was essential for high affinity binding to the human B1 receptor. In marked contrast to cloned Chinese hamster ovary cells expressing the human kinin B2 receptor, which internalized approximately 80% of the ligand within 5 min upon exposure to 2 nM [3H]bradykinin, exposure of cells expressing the B1 receptor to 1 nM [3H]des-Arg10-lysylbradykinin resulted in minimal ligand internalization. Stimulation of the B1 receptor led to inositol phosphate generation and transient increases in intracellular calcium, confirming coupling to phospholipase C, while immunoprecipitation of photoaffinity-labeled G-proteins from membranes indicated specific coupling of the receptor to Galphaq/11 and Galphai1,2. The B1, unlike the B2, receptor does not desensitize (as demonstrated by continuous phosphoinositide hydrolysis), enhancing the potential role of this receptor during inflammatory events.

摘要

为了描绘人B1激肽受体的配体结合和功能特性,分离出了一个稳定的中国仓鼠卵巢细胞克隆,该克隆表达一类对[3H]去-Arg10-赖氨酰缓激肽具有单一结合位点,解离常数(Kd)为0.3 nM,最大结合量(Bmax)为38 fmol/mg蛋白(约40,000个受体/细胞)。对肽类似物的研究表明,配体第1位(基于赖氨酰缓激肽序列)的赖氨酸残基对于与人B1受体的高亲和力结合至关重要。与表达人激肽B2受体的克隆中国仓鼠卵巢细胞形成显著对比,后者在暴露于2 nM [3H]缓激肽后5分钟内可内化约80%的配体,而将表达B1受体的细胞暴露于1 nM [3H]去-Arg10-赖氨酰缓激肽后,配体内化极少。对B1受体的刺激导致肌醇磷酸生成以及细胞内钙的短暂增加,证实其与磷脂酶C偶联,同时从膜上免疫沉淀光亲和标记的G蛋白表明该受体与Gαq/11和Gαi1,2特异性偶联。与B2受体不同,B1受体不会脱敏(如持续的磷酸肌醇水解所示),这增强了该受体在炎症事件中的潜在作用。

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