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P物质(NK-1)受体与G蛋白Gq和G11的α亚基的化学交联。

Chemical cross-linking of the substance P (NK-1) receptor to the alpha subunits of the G proteins Gq and G11.

作者信息

Macdonald S G, Dumas J J, Boyd N D

机构信息

Department of Pharmacology and Experimental Therapeutics, Boston University School of Medicine, Massachusetts 02118, USA.

出版信息

Biochemistry. 1996 Mar 5;35(9):2909-16. doi: 10.1021/bi952351+.

Abstract

We have previously shown that the high-affinity binding of substance P (SP) to its receptor is dependent on an interaction with a PTX-insensitive G protein. This G protein couples SP receptor activation to stimulation of its effector, phospholipase C. In this study, we combined photoaffinity labeling, chemical cross-linking techniques, and immunological characterization using sequence-specific antibody probes to identify G proteins that couple to the SP receptor. First we covalently labeled the SP receptor present on rat submaxillary gland membranes with a radioiodinated photoreactive derivative of SP, p-benzoyl-L-phenylalanine(8)-substance P (125I-[Bpa8]SP). Photoincorporation of this SP derivative was susceptible to guanine nucleotide inhibition, indicating that the receptor was coupled to its G protein during labeling. We then used a chemical cross-linking agent to covalently link the photoaffinity labeled SP receptor and its associated G protein. Cross-linking generated a 96 kDa product, formation of which was prevented by the addition of a guanine nucleotide, but not an adenine nucleotide, following photolabeling, but prior to cross-linking. Furthermore, the 96 kDa cross-linked complex was absent in membranes which had been depleted of G proteins by treatment with alkaline buffer prior to addition of the cross-linking agent. Reductive cleavage of the cross-link in the isolated 96 kDa complex yields two products: the 53 kDa SP receptor and a 42 kDa protein identified by immunoblot analysis as either G alpha q or G alpha 11. Antisera against a common sequence within G alpha s, G alpha i, and G alpha o showed no immunoreactivity to the complex or its cleavage products. These results provide the first direct evidence of specific interaction between photoaffinity labeled SP receptor and the alpha subunits of Gq and G11, members of a family of G proteins known to be associated with pertussis toxin-insensitive phospholipase C activation.

摘要

我们先前已表明,P物质(SP)与其受体的高亲和力结合依赖于与一种对百日咳毒素(PTX)不敏感的G蛋白的相互作用。这种G蛋白将SP受体激活与其效应器磷脂酶C的刺激偶联起来。在本研究中,我们结合了光亲和标记、化学交联技术以及使用序列特异性抗体探针的免疫学表征,以鉴定与SP受体偶联的G蛋白。首先,我们用SP的放射性碘化光反应性衍生物对苯甲酰-L-苯丙氨酸(8)-P物质(125I-[Bpa8]SP)共价标记大鼠颌下腺膜上存在的SP受体。这种SP衍生物的光掺入易受鸟嘌呤核苷酸抑制,表明在标记过程中受体与其G蛋白偶联。然后我们使用一种化学交联剂将光亲和标记的SP受体及其相关的G蛋白共价连接起来。交联产生了一种96 kDa的产物,在光标记后但交联前加入鸟嘌呤核苷酸而非腺嘌呤核苷酸可阻止该产物形成。此外,在用交联剂处理前用碱性缓冲液耗尽G蛋白的膜中不存在96 kDa的交联复合物。对分离的96 kDa复合物中的交联进行还原性切割产生两种产物:53 kDa的SP受体和通过免疫印迹分析鉴定为Gαq或Gα11的42 kDa蛋白。针对Gαs、Gαi和Gαo内共同序列的抗血清对该复合物或其切割产物无免疫反应性。这些结果首次直接证明了光亲和标记的SP受体与Gq和G11的α亚基之间存在特异性相互作用,Gq和G11是已知与百日咳毒素不敏感的磷脂酶C激活相关的G蛋白家族成员。

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