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α1C基因的可变剪接IS6片段决定了心脏和血管平滑肌L型Ca2+通道的组织特异性二氢吡啶敏感性。

Alternatively spliced IS6 segments of the alpha 1C gene determine the tissue-specific dihydropyridine sensitivity of cardiac and vascular smooth muscle L-type Ca2+ channels.

作者信息

Welling A, Ludwig A, Zimmer S, Klugbauer N, Flockerzi V, Hofmann F

机构信息

Institut für Pharmakologie und Toxikologie der Technischen Universität München, Germany.

出版信息

Circ Res. 1997 Oct;81(4):526-32. doi: 10.1161/01.res.81.4.526.

Abstract

Dihydropyridines (DHPs) block the vascular smooth muscle L-type Ca2+ channel at lower concentrations than the cardiac Ca2+ channel, although their alpha 1 subunit, which binds the DHPs, is derived from the same gene. This alpha 1C gene gives rise to several splice variants, among which the alpha 1C-b variant is affected by lower concentrations of nisoldipine than the alpha 1C-a variant. Functional expression of chimeras of alpha 1C-a and alpha 1C-b subunits demonstrated that the transmembrane segment IS6 is responsible for the different dihydropyridine sensitivity. Northern blot analysis showed that transcripts coding for the IS6 segment of the alpha 1C-a subunit were expressed in heart but not in aorta, whereas the IS6 segment of the alpha 1C-b subunit was expressed predominantly in vascular smooth muscle. In situ hybridization of rat heart sections confirmed this expression pattern of IS6 alpha 1C-a and IS6 alpha 1C-b in ventricular and smooth muscle myocytes, respectively. These results suggest that the different dihydropyridine sensitivities of cardiac and vascular L-type Ca2+ channels are caused at least partially by the tissue-specific expression of alternatively spliced IS6 segments of the alpha 1C gene.

摘要

二氢吡啶类(DHPs)在比心脏钙通道更低的浓度下就能阻断血管平滑肌L型钙通道,尽管它们与二氢吡啶类结合的α1亚基来自同一个基因。这个α1C基因产生了几种剪接变体,其中α1C - b变体比α1C - a变体对尼索地平的浓度更低就有反应。α1C - a和α1C - b亚基嵌合体的功能表达表明,跨膜片段IS6是造成二氢吡啶敏感性差异的原因。Northern印迹分析显示,编码α1C - a亚基IS6片段的转录本在心脏中表达,但在主动脉中不表达,而α1C - b亚基的IS6片段主要在血管平滑肌中表达。大鼠心脏切片的原位杂交证实了IS6 α1C - a和IS6 α1C - b分别在心室肌细胞和平滑肌细胞中的这种表达模式。这些结果表明,心脏和血管L型钙通道对二氢吡啶敏感性的差异至少部分是由α1C基因可变剪接的IS6片段的组织特异性表达所导致的。

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