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通过卵母细胞表达系统克隆牛速激肽K受体的cDNA

cDNA cloning of bovine substance-K receptor through oocyte expression system.

作者信息

Masu Y, Nakayama K, Tamaki H, Harada Y, Kuno M, Nakanishi S

机构信息

Institute for Immunology, Kyoto University Faculty of Medicine, Japan.

出版信息

Nature. 1987;329(6142):836-8. doi: 10.1038/329836a0.

Abstract

The neuropeptide receptors which are present in very small quantities in the cell and are embedded tightly in the plasma membrane have not been well characterized. Mammals contain three distinct tachykinin neuropeptides, substance P, substance K and neuromedin K, and it has been suggested that there are multiple tachykinin receptors. By electrophysiological measurement, we have previously shown that Xenopus oocytes injected with brain and stomach mRNAs faithfully express mammalian substance-P and substance-K receptors, respectively. Here we report the isolation of the cDNA clone for bovine substance-K receptor (SKR) by extending this method to develop a new cloning strategy. We constructed a stomach cDNA library with a cloning vector that allowed in vitro synthesis of mRNAs and then identified a particular cDNA clone by testing for receptor expression following injection of the mRNAs synthesized in vitro into the oocyte system. Because oocytes injected with exogenous mRNAs can express numerous receptors and channels, our new strategy will be applicable in the general molecular cloning of these proteins. The result provides the first indication that the neuropeptide receptor has sequence similarity with rhodopsin-type receptors (the G-protein-coupled receptor family) and thus possesses multiple membrane-spanning domains.

摘要

细胞中含量极少且紧密嵌入质膜的神经肽受体尚未得到充分表征。哺乳动物含有三种不同的速激肽神经肽,即P物质、K物质和神经介素K,有人认为存在多种速激肽受体。通过电生理测量,我们先前已表明,注射了脑和胃mRNA的非洲爪蟾卵母细胞分别忠实地表达了哺乳动物的P物质和K物质受体。在此,我们报告通过扩展该方法以开发新的克隆策略来分离牛K物质受体(SKR)的cDNA克隆。我们用一种允许体外合成mRNA的克隆载体构建了胃cDNA文库,然后通过将体外合成的mRNA注射到卵母细胞系统中检测受体表达来鉴定特定的cDNA克隆。由于注射外源mRNA的卵母细胞可表达众多受体和通道,我们的新策略将适用于这些蛋白质的一般分子克隆。结果首次表明该神经肽受体与视紫红质型受体(G蛋白偶联受体家族)具有序列相似性,因此具有多个跨膜结构域。

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