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大鼠脑和神经内分泌GH3细胞表达的Cav1.3(α1D)L型钙通道剪接变体的功能特性

Functional properties of Cav1.3 (alpha1D) L-type Ca2+ channel splice variants expressed by rat brain and neuroendocrine GH3 cells.

作者信息

Safa P, Boulter J, Hales T G

机构信息

Department of Pharmacology, The George Washington University, Washington, DC 20037, USA.

出版信息

J Biol Chem. 2001 Oct 19;276(42):38727-37. doi: 10.1074/jbc.M103724200. Epub 2001 Aug 20.

DOI:10.1074/jbc.M103724200
PMID:11514547
Abstract

Ca(2+) enters pituitary and pancreatic neuroendocrine cells through dihydropyridine-sensitive channels triggering hormone release. Inhibitory metabotropic receptors reduce Ca(2+) entry through activation of pertussis toxin-sensitive G proteins leading to activation of K(+) channels and voltage-sensitive inhibition of L-type channel activity. Despite the cloning and functional expression of several Ca(2+) channels, those involved in regulating hormone release remain unknown. Using reverse transcription-polymerase chain reaction we identified mRNAs encoding three alpha(1) (alpha(1A), alpha(1C), and alpha(1D)), four beta, and one alpha(2)-delta subunit in rat pituitary GH(3) cells; alpha(1B) and alpha(1S) transcripts were absent. GH(3) cells express multiple alternatively spliced alpha(1D) mRNAs. Many of the alpha(1D) transcript variants encode "short" alpha(1D) (alpha(1D-S)) subunits, which have a QXXER amino acid sequence at their C termini, a motif found in all other alpha(1) subunits that couple to opioid receptors. The other splice variants identified terminate with a longer C terminus that lacks the QXXER motif (alpha(1D-L)). We cloned and expressed the predominant alpha(1D-S) transcript variants in rat brain and GH(3) cells and their alpha(lD-L) counterpart in GH(3) cells. Unlike alpha(1A) channels, alpha(1D) channels exhibited current-voltage relationships similar to those of native GH(3) cell Ca(2+) channels, but lacked voltage-dependent G protein coupling. Our data demonstrate that alternatively spliced alpha(1D) transcripts form functional Ca(2+) channels that exhibit voltage-dependent, G protein-independent facilitation. Furthermore, the QXXER motif, located on the C terminus of alpha(1D-S) subunit, is not sufficient to confer sensitivity to inhibitory G proteins.

摘要

钙离子通过对二氢吡啶敏感的通道进入垂体和胰腺神经内分泌细胞,触发激素释放。抑制性代谢型受体通过激活百日咳毒素敏感的G蛋白减少钙离子内流,导致钾通道激活以及L型通道活性的电压敏感性抑制。尽管已经克隆并功能性表达了几种钙离子通道,但参与调节激素释放的通道仍不清楚。我们利用逆转录-聚合酶链反应在大鼠垂体GH(3)细胞中鉴定出编码三个α(1)(α(1A)、α(1C)和α(1D))、四个β和一个α(2)-δ亚基的mRNA;未检测到α(1B)和α(1S)转录本。GH(3)细胞表达多种选择性剪接的α(1D)mRNA。许多α(1D)转录本变体编码“短”α(1D)(α(1D-S))亚基,其C末端具有QXXER氨基酸序列,该基序存在于所有与阿片受体偶联的其他α(1)亚基中。鉴定出的其他剪接变体以缺乏QXXER基序的较长C末端终止(α(1D-L))。我们在大鼠脑和GH(3)细胞中克隆并表达了主要的α(1D-S)转录本变体以及在GH(3)细胞中的α(1D-L)对应物。与α(1A)通道不同,α(1D)通道表现出与天然GH(3)细胞钙离子通道相似的电流-电压关系,但缺乏电压依赖性G蛋白偶联。我们的数据表明,选择性剪接的α(1D)转录本形成功能性钙离子通道,表现出电压依赖性、不依赖G蛋白的易化作用。此外,位于α(1D-S)亚基C末端的QXXER基序不足以赋予对抑制性G蛋白的敏感性。

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