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心房利钠肽清除受体。cDNA克隆的完整序列及功能表达。

Atrial natriuretic peptide clearance receptor. Complete sequence and functional expression of cDNA clones.

作者信息

Fuller F, Porter J G, Arfsten A E, Miller J, Schilling J W, Scarborough R M, Lewicki J A, Schenk D B

机构信息

California Biotechnology, Inc., Mountain View 94043.

出版信息

J Biol Chem. 1988 Jul 5;263(19):9395-401.

PMID:2837487
Abstract

The major class of atrial natriuretic peptide (ANP) receptors was isolated from cultured vascular smooth muscle cells, and a partial amino acid sequence was obtained. This allowed the isolation of cDNA clones from which the entire amino acid sequence was established. The smooth muscle cell ANP receptor appears to be synthesized as a 537-amino acid precursor with an N-terminal membrane translocation signal. The mature form consists of 496 amino acids with a single potential transmembrane domain predicting a 37-amino acid cytoplasmic domain and a large, acidic, extracellular domain low in cysteine and probably containing attached carbohydrate. The receptor is therefore similar in structure to the growth factor receptors but notably lacks repetitive cysteine-rich domains and has a relatively small intracellular domain. Expression of the cloned receptor in Xenopus oocytes elicited high affinity, membrane-associated binding sites for ANP and for truncated and internally deleted analogs of ANP. These results reflect the ligand binding specificity found for the major class of ANP receptors on smooth muscle cells and thus provide additional evidence that two distinct ANP receptors exist since ANP receptor-coupled guanylate cyclase activity exhibits a very different ANP analog specificity.

摘要

心房利钠肽(ANP)受体的主要类别是从培养的血管平滑肌细胞中分离出来的,并获得了部分氨基酸序列。这使得能够分离出cDNA克隆,据此确定了完整的氨基酸序列。平滑肌细胞ANP受体似乎是以一种含537个氨基酸的前体形式合成的,其N端具有膜转运信号。成熟形式由496个氨基酸组成,有一个潜在的单一跨膜结构域,预测有一个37个氨基酸的胞质结构域和一个大的、酸性的、半胱氨酸含量低且可能含有连接碳水化合物的细胞外结构域。因此,该受体在结构上与生长因子受体相似,但明显缺乏富含半胱氨酸的重复结构域,且细胞内结构域相对较小。在非洲爪蟾卵母细胞中克隆受体的表达引发了对ANP以及ANP的截短和内部缺失类似物的高亲和力、膜相关结合位点。这些结果反映了在平滑肌细胞上主要类别ANP受体的配体结合特异性,因此提供了额外证据,证明存在两种不同的ANP受体,因为ANP受体偶联的鸟苷酸环化酶活性表现出非常不同的ANP类似物特异性。

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