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一种新型人类神经激肽-3受体同源物的功能表达,该同源物可结合[³H]senktide和[¹²⁵I-MePhe⁷]神经激肽B,并对速激肽肽激动剂有反应。

Functional expression of a novel human neurokinin-3 receptor homolog that binds [3H]senktide and [125I-MePhe7]neurokinin B, and is responsive to tachykinin peptide agonists.

作者信息

Krause J E, Staveteig P T, Mentzer J N, Schmidt S K, Tucker J B, Brodbeck R M, Bu J Y, Karpitskiy V V

机构信息

Department of Anatomy and Neurobiology, Washington University School of Medicine, St. Louis, MO 63110, USA.

出版信息

Proc Natl Acad Sci U S A. 1997 Jan 7;94(1):310-5. doi: 10.1073/pnas.94.1.310.

Abstract

In 1992, Xie et al. identified a cDNA sequence in the expression cloning search for the kappa opioid receptor. When the cDNA was expressed in Cos-7 cells, binding of opioid compounds was observed to be of low affinity and without kappa, mu, or delta selectivity [Xie, G.-X., Miyajima, A. and Goldstein, A. (1992) Proc. Natl. Acad. Sci. USA 89, 4124-4128]. This cDNA was highly homologous to the human neurokinin-3 (NK-3) receptor sequence, and displayed lower homology to NK-1 and NK-2 sequences. This sequence was stably expressed in Chinese hamster ovary cells, which do not express neurokinin receptors naturally, and ligand binding and second messenger characteristics were compared with a human NK-3 receptor. The NK-3 receptor homolog bound [3H] senktide with a Kd of 39 nM, similar to that of the NK-3 receptor. The rank order of tachykinin peptides competing for [3H]senktide binding at the NK-3 receptor homolog was [MePhe7]neurokinin B > senktide > substance P = neurokinin A > neurokinin B. This cell line also bound [125I-MePhe7]neurokinin B; however, neurokinin B was an effective competitor. Tachykinin peptides stimulated both inositol phospholipid hydrolysis and arachidonic acid release at NK-3 and NK-3 receptor homolog cell lines, with similar rank orders of potency of [MePhe7] neurokinin B = neurokinin B = senktide > NKA = substance P. These results indicate that expression of the NK-3 receptor homolog cDNA in the Chinese hamster ovary cell system induces the expression of a receptor site with many similarities but certain key differences from that of the human NK-3 receptor. The results are discussed with reference to the existence of a novel human tachykinin receptor.

摘要

1992年,谢等人在表达克隆研究中鉴定出一种与κ阿片受体相关的cDNA序列。当该cDNA在Cos-7细胞中表达时,观察到阿片类化合物的结合具有低亲和力,且对κ、μ或δ受体无选择性[谢,G.-X.,宫岛,A.和戈尔茨坦,A.(1992年)《美国国家科学院院刊》89,4124 - 4128]。该cDNA与人神经激肽-3(NK-3)受体序列高度同源,与NK-1和NK-2序列的同源性较低。该序列在中国仓鼠卵巢细胞中稳定表达,这些细胞天然不表达神经激肽受体,并将配体结合和第二信使特征与人NK-3受体进行了比较。NK-3受体同源物与[3H]速激肽的结合解离常数(Kd)为39 nM,与NK-3受体相似。在NK-3受体同源物上竞争[3H]速激肽结合的速激肽肽段的活性顺序为:[MePhe7]神经激肽B > 速激肽 > P物质 = 神经激肽A > 神经激肽B。该细胞系也能结合[125I-MePhe7]神经激肽B;然而,神经激肽B是一种有效的竞争剂。速激肽肽段在NK-3和NK-3受体同源物细胞系中均刺激肌醇磷脂水解和花生四烯酸释放,其活性顺序相似为:[MePhe7]神经激肽B = 神经激肽B = 速激肽 > NKA = P物质。这些结果表明,NK-3受体同源物cDNA在中国仓鼠卵巢细胞系统中的表达诱导了一种受体位点的表达,该受体位点与人类NK-3受体有许多相似之处,但也存在某些关键差异。结合一种新型人类速激肽受体的存在对这些结果进行了讨论。

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