Lee T W, Anderson L A, Eidne K A, Milligan G
Division of Biochemistry and Molecular Biology, University of Glasgow, Scotland, U.K.
Biochem J. 1995 Aug 15;310 ( Pt 1)(Pt 1):291-8. doi: 10.1042/bj3100291.
cDNA species encoding either the long or the short isoforms of the rat thyrotropin-releasing-hormone (TRH) receptor were expressed stably in Rat 1 fibroblasts, and clones expressing specific binding of [3H]TRH were detected and expanded. Clones expressing each of these receptors at levels up to 1 pmol/mg of membrane protein were selected for analysis. Reverse-transcriptase PCR on RNA isolated from these clones confirmed that each clone expressed only mRNA corresponding to the expected splice variant. Both receptor splice variants bound [3H]TRH with a Kd of some 80 nM when binding assays were performed in the presence of guanosine 5'-[beta gamma-imido]-triphosphate. In the presence of TRH, both receptor subtypes were able to cause stimulation of inositol phosphate generation in a pertussis-toxin-insensitive manner with similar EC50 values and to stimulate the mobilization of intracellular Ca2+, but, despite reports that TRH receptors can also interact with the G-proteins Gs and Gi2, neither receptor splice variant was able to modulate adenylate cyclase activity in either a positive or a negative manner. These data indicate that the long and short isoforms of the rat TRH receptor have similar affinities for TRH and display similar abilities to interact with the Gq-like G-proteins, but show no ability to regulate adenylate cyclase, at least when expressed in this genetic background.
编码大鼠促甲状腺激素释放激素(TRH)受体长亚型或短亚型的cDNA在大鼠1成纤维细胞中稳定表达,检测并扩增出表达[3H]TRH特异性结合的克隆。选择膜蛋白水平高达1 pmol/mg时表达这些受体的克隆进行分析。对从这些克隆中分离的RNA进行逆转录酶PCR证实,每个克隆仅表达对应于预期剪接变体的mRNA。当在鸟苷5'-[βγ-亚氨基] -三磷酸存在下进行结合测定时,两种受体剪接变体均以约80 nM的Kd结合[3H]TRH。在TRH存在下,两种受体亚型均能够以百日咳毒素不敏感的方式刺激肌醇磷酸生成,具有相似的EC50值,并刺激细胞内Ca2+的动员,但是,尽管有报道称TRH受体也可与G蛋白Gs和Gi2相互作用,但两种受体剪接变体均不能以正向或负向方式调节腺苷酸环化酶活性。这些数据表明,大鼠TRH受体的长亚型和短亚型对TRH具有相似的亲和力,并表现出与Gq样G蛋白相互作用的相似能力,但至少在这种遗传背景下表达时,没有调节腺苷酸环化酶的能力。
