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培养的大鼠小胶质细胞中腺苷 A2a 受体刺激对钾离子通道 mRNA 表达的调控

Regulation of K+ channel mRNA expression by stimulation of adenosine A2a-receptors in cultured rat microglia.

作者信息

Küst B M, Biber K, van Calker D, Gebicke-Haerter P J

机构信息

Institute for Biology III, University of Freiburg, Germany.

出版信息

Glia. 1999 Jan 15;25(2):120-30.

PMID:9890627
Abstract

Previous investigations suggest that the expression of K+ channels in cultured rat microglia is related to the activation status of these cells. Both, lipopolysaccharide (LPS) and agents that raise intracellular cyclic AMP have been shown to inhibit microglial proliferation. LPS also regulates the mRNA expression levels of K+ channels in cultured microglia, which led us to investigate possible regulatory interactions between K+ channels and adenosine A2a-receptors, which are coupled to the cAMP-signal transduction pathway. The selective adenosine A2a-receptor agonist CGS 21680 induced enhanced mRNA expression of both Kv1.3 and ROMK1, as well as an elevation of Kv1.3 protein. The selective adenosine A2a-receptor antagonist aminophenol (ZM 241385) and the nonselective antagonist 8-phenyltheophylline (8-PT) inhibited these effects. Elevations of cyclic AMP by use of dibutyryl cyclic AMP (dbcAMP), phosphodiesterase-inhibitor (RO 20-1724), forskolin, or cholera toxin (CTX), strongly enhanced Kv1.3-mRNA expression, but decreased ROMK1-mRNA levels. Results from experiments with actinomycin D suggest that K+ channel mRNA levels in cultured microglia were regulated by altered mRNA synthesis. Evidently, the CGS 21680-induced effects upon Kv1.3 were mediated via an increase in intracellular cyclic AMP, whereas ROMK1-mRNA expression appeared to be regulated by coupling of adenosine A2a-receptors to an alternative pathway, which involves activation of protein kinase C (PKC). It is concluded that the cyclic AMP second messenger system in microglia is not only involved in regulation of K+ channel activity, but also in regulation of de novo K+ channel synthesis.

摘要

先前的研究表明,培养的大鼠小胶质细胞中钾离子通道的表达与这些细胞的激活状态有关。脂多糖(LPS)和提高细胞内环磷酸腺苷(cAMP)的物质均已显示可抑制小胶质细胞增殖。LPS还调节培养的小胶质细胞中钾离子通道的mRNA表达水平,这促使我们研究钾离子通道与腺苷A2a受体之间可能的调节相互作用,腺苷A2a受体与cAMP信号转导途径偶联。选择性腺苷A2a受体激动剂CGS 21680可诱导Kv1.3和ROMK1的mRNA表达增强,以及Kv1.3蛋白水平升高。选择性腺苷A2a受体拮抗剂氨苯酚(ZM 241385)和非选择性拮抗剂8-苯基茶碱(8-PT)可抑制这些作用。通过使用二丁酰环磷酸腺苷(dbcAMP)、磷酸二酯酶抑制剂(RO 20-1724)、福斯可林或霍乱毒素(CTX)提高cAMP水平,可强烈增强Kv1.3-mRNA表达,但降低ROMK1-mRNA水平。放线菌素D实验结果表明,培养的小胶质细胞中钾离子通道mRNA水平受mRNA合成变化的调节。显然,CGS 21680对Kv1.3的诱导作用是通过细胞内环磷酸腺苷增加介导的,而ROMK1-mRNA表达似乎是由腺苷A2a受体与另一条途径偶联调节的,该途径涉及蛋白激酶C(PKC)的激活。结论是,小胶质细胞中的环磷酸腺苷第二信使系统不仅参与钾离子通道活性的调节,还参与钾离子通道从头合成的调节。

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