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半胱氨酸18-半胱氨酸274二硫键及第三个细胞外环在血管紧张素II 1型受体组成性激活和内化中的作用

Role of the Cys18-Cys274 disulfide bond and of the third extracellular loop in the constitutive activation and internalization of angiotensin II type 1 receptor.

作者信息

Correa Silvana A A, Pignatari Graciela C, Ferro Emer S, Pacheco Nelson A S, Costa-Neto Claudio M, Pesquero João B, Oliveira Laerte, Paiva Antonio C M, Shimuta Suma I

机构信息

Department of Biophysics, Universidade Federal de São Paulo-Escola Paulista de Medicina, Rua Botucatu 862, 04023-062, São Paulo, SP, Brazil.

出版信息

Regul Pept. 2006 May 15;134(2-3):132-40. doi: 10.1016/j.regpep.2006.02.008. Epub 2006 Apr 19.

DOI:10.1016/j.regpep.2006.02.008
PMID:16626818
Abstract

An insertion of residues in the third extracellular loop and a disulfide bond linking this loop to the N-terminal domain were identified in a structural model of a G-protein coupled receptor specific to angiotensin II (AT1 receptor), built in homology to the seven-transmembrane-helix bundle of rhodopsin. Both the insertion and the disulfide bond were located close to an extracellular locus, flanked by the second extracellular loop (EC-2), the third extracellular loop (EC-3) and the N-terminal domain of the receptor; they contained residues identified by mutagenesis studies to bind the angiotensin II N-terminal segment (residues D1 and R2). It was postulated that the insertion and the disulfide bond, also found in other receptors such as those for bradykinin, endothelin, purine and other ligands, might play a role in regulating the function of the AT1 receptor. This possibility was investigated by assaying AT1 forms devoid of the insertion and with mutations to Ser on both positions of Cys residues forming the disulfide bond. Binding and activation experiments showed that abolition of this bond led to constitutive activation, decay of agonist binding and receptor activation levels. Furthermore, the receptors thus mutated were translocated to cytosolic environments including those in the nucleus. The receptor form with full deletion of the EC-3 loop residue insertion, displayed a wild type receptor behavior.

摘要

在一个与视紫红质的七跨膜螺旋束具有同源性构建的、针对血管紧张素 II 的 G 蛋白偶联受体(AT1 受体)的结构模型中,发现了第三个细胞外环中存在残基插入,以及一个将该环与 N 端结构域相连的二硫键。插入片段和二硫键均位于靠近一个细胞外位点处,该位点两侧为受体的第二个细胞外环(EC - 2)、第三个细胞外环(EC - 3)和 N 端结构域;它们包含通过诱变研究确定的与血管紧张素 II N 端片段(残基 D1 和 R2)结合的残基。据推测,在其他受体如缓激肽、内皮素、嘌呤及其他配体的受体中也发现的这种插入片段和二硫键,可能在调节 AT1 受体的功能中发挥作用。通过检测缺失插入片段以及形成二硫键的半胱氨酸残基两个位置均突变为丝氨酸后的 AT1 形式来研究这种可能性。结合和激活实验表明,去除该二硫键会导致组成性激活、激动剂结合能力下降以及受体激活水平降低。此外,如此突变后的受体转移至包括细胞核内的胞质环境中。完全缺失 EC - 3 环残基插入的受体形式表现出野生型受体行为。

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