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核α1 - 肾上腺素能受体信号激活成年心肌细胞中细胞外调节蛋白激酶(ERK)定位于小窝。

Nuclear alpha1-adrenergic receptors signal activated ERK localization to caveolae in adult cardiac myocytes.

作者信息

Wright Casey D, Chen Quanhai, Baye Nichole L, Huang Yuan, Healy Chastity L, Kasinathan Sivakanthan, O'Connell Timothy D

机构信息

Cardiovascular Research Center, Sanford Research/USD, Sioux Falls, SD 57105, USA.

出版信息

Circ Res. 2008 Oct 24;103(9):992-1000. doi: 10.1161/CIRCRESAHA.108.176024. Epub 2008 Sep 18.

Abstract

We previously identified an alpha1-AR-ERK (alpha1A-adrenergic receptor-extracellular signal-regulated kinase) survival signaling pathway in adult cardiac myocytes. Here, we investigated localization of alpha1-AR subtypes (alpha1A and alpha1B) and how their localization influences alpha1-AR signaling in cardiac myocytes. Using binding assays on myocyte subcellular fractions or a fluorescent alpha1-AR antagonist, we localized endogenous alpha1-ARs to the nucleus in wild-type adult cardiac myocytes. To clarify alpha1 subtype localization, we reconstituted alpha1 signaling in cultured alpha1A- and alpha1B-AR double knockout cardiac myocytes using alpha1-AR-green fluorescent protein (GFP) fusion proteins. Similar to endogenous alpha1-ARs and alpha1A- and alpha1B-GFP colocalized with LAP2 at the nuclear membrane. alpha1-AR nuclear localization was confirmed in vivo using alpha1-AR-GFP transgenic mice. The alpha1-signaling partners Galphaq and phospholipase Cbeta1 also colocalized with alpha1-ARs only at the nuclear membrane. Furthermore, we observed rapid catecholamine uptake mediated by norepinephrine-uptake-2 and found that alpha1-mediated activation of ERK was not inhibited by a membrane impermeant alpha1-blocker, suggesting alpha1 signaling is initiated at the nucleus. Contrary to prior studies, we did not observe alpha1-AR localization to caveolae, but we found that alpha1-AR signaling initiated at the nucleus led to activated ERK localized to caveolae. In summary, our results show that nuclear alpha1-ARs transduce signals to caveolae at the plasma membrane in cardiac myocytes.

摘要

我们之前在成年心肌细胞中鉴定出一条α1-AR-ERK(α1A-肾上腺素能受体-细胞外信号调节激酶)存活信号通路。在此,我们研究了α1-AR亚型(α1A和α1B)的定位以及它们的定位如何影响心肌细胞中的α1-AR信号传导。通过对心肌细胞亚细胞组分进行结合测定或使用荧光α1-AR拮抗剂,我们将野生型成年心肌细胞中的内源性α1-AR定位到细胞核。为了阐明α1亚型的定位,我们使用α1-AR-绿色荧光蛋白(GFP)融合蛋白在培养的α1A-和α1B-AR双敲除心肌细胞中重建α1信号传导。与内源性α1-AR相似,α1A-和α1B-GFP在核膜处与LAP2共定位。使用α1-AR-GFP转基因小鼠在体内证实了α1-AR的核定位。α1信号传导伙伴Gαq和磷脂酶Cβ1也仅在核膜处与α1-AR共定位。此外,我们观察到去甲肾上腺素摄取-2介导的快速儿茶酚胺摄取,并发现α1介导的ERK激活不受膜不透性α1阻滞剂的抑制,表明α1信号传导在细胞核处起始。与先前的研究相反,我们未观察到α1-AR定位于小窝,但我们发现细胞核处起始的α1-AR信号传导导致活化的ERK定位于小窝。总之,我们的结果表明,核α1-AR在心肌细胞中将信号转导至质膜上的小窝。

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