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Giα2在体内介导对腺苷酸环化酶的抑制性调节:在可诱导反义RNA抑制Giα2的转基因小鼠中的分析。

Gi alpha 2 mediates the inhibitory regulation of adenylylcyclase in vivo: analysis in transgenic mice with Gi alpha 2 suppressed by inducible antisense RNA.

作者信息

Moxham C M, Hod Y, Malbon C C

机构信息

Department of Molecular Pharmacology, State University of New York at Stony Brook 11794-8651.

出版信息

Dev Genet. 1993;14(4):266-73. doi: 10.1002/dvg.1020140404.

DOI:10.1002/dvg.1020140404
PMID:7693386
Abstract

The role of the GTP-binding regulatory protein (G-protein) Gi alpha 2 in vivo was explored using transgenic mice in which the alpha-subunit of Gi alpha 2 was suppressed by antisense RNA. Rat hepatoma FTO-2B cells provide an ideal test system for constructs employing the expression vector pPCK-AS, designed to express antisense RNA at birth under the control of the phosphoenolpyruvate carboxykinase (PEPCK) promoter. Cells transfected with the expression vector containing a sequence antisense to Gi alpha 2 (pPCK-ASGi alpha 2) displayed expression of RNA antisense to Gi alpha 2 that, like transcription of the PEPCK gene, was inducible by cyclic AMP. Expression of RNA antisense to Gi alpha 2 and suppression of the expression of Gi alpha 2, but not Gsa and Gi alpha 3, was observed in the transfected FTO-2B cells. BDF1 mice carrying the transgene displayed suppression of Gi alpha 2 in liver and fat, two targets for tissue-specific expression of the PEPCK gene. The loss of Gi alpha 2 in white adipocytes of transgenic mice resulted in 3.1-fold elevation of basal cyclic AMP accumulation. Cyclic AMP accumulation in response to stimulation by epinephrine (10 microM) was normal in adipocytes of transgenic mice, demonstrating no alteration in the stimulatory adenylylcyclase capacity in the Gi alpha 2-deficient cells. The inhibitory adenylylcyclase pathway, in sharp contrast, was severely blunted in response to challenge by the inhibitory A1-purinergic agonist, (-)R-N6-phenylisopropyladenosine. These studies illuminate a critical role of Gi alpha 2 in the inhibitory adenylylcyclase signaling pathway in vivo.

摘要

利用转基因小鼠探索了GTP结合调节蛋白(G蛋白)Giα2在体内的作用,在这些小鼠中,Giα2的α亚基被反义RNA抑制。大鼠肝癌FTO - 2B细胞为采用表达载体pPCK - AS的构建体提供了理想的测试系统,该载体设计为在磷酸烯醇丙酮酸羧激酶(PEPCK)启动子的控制下在出生时表达反义RNA。用含有与Giα2反义序列的表达载体(pPCK - ASGiα2)转染的细胞显示出对Giα2反义RNA的表达,该反义RNA与PEPCK基因的转录一样,可被环磷酸腺苷诱导。在转染的FTO - 2B细胞中观察到了对Giα2反义RNA的表达以及Giα2表达的抑制,但未观察到Gsα和Giα3表达的抑制。携带转基因的BDF1小鼠在肝脏和脂肪中显示出Giα2的抑制,肝脏和脂肪是PEPCK基因组织特异性表达的两个靶点。转基因小鼠白色脂肪细胞中Giα2的缺失导致基础环磷酸腺苷积累升高3.1倍。转基因小鼠脂肪细胞中对肾上腺素(10μM)刺激的环磷酸腺苷积累正常,表明Giα2缺陷细胞中刺激性腺苷酸环化酶能力未改变。与之形成鲜明对比的是,抑制性腺苷酸环化酶途径在受到抑制性A1 - 嘌呤能激动剂( - )R - N6 - 苯基异丙基腺苷刺激时严重减弱。这些研究阐明了Giα2在体内抑制性腺苷酸环化酶信号通路中的关键作用。

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