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首页> 外文期刊>Experimental Biology and Medicine: Journal of the Society for Experimental Biology and Medicine >RNA transfection is a versatile tool to investigate endothelin-1 posttranscriptional regulation.
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RNA transfection is a versatile tool to investigate endothelin-1 posttranscriptional regulation.

机译:RNA转染是研究内皮素-1转录后调控的多功能工具。

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Endothelin-1 (ET-1) is a potent endothelial-derived vasoconstrictor and cellular mitogen. Perturbations in ET-1 levels have been observed in a number of cardiovascular and renal disorders. Steady-state ET-1 mRNA expression is regulated in the vascular endothelium by an inducible promoter and a constitutively short mRNA half-life. Recent studies have identified mRNA stabilization as a pathophysiologically relevant mechanism of ET-1 induction in vascular endothelial cells. However, mechanistic studies on posttranscriptional pathways in physiologically relevant postconfluent primary endothelial cell monolayers have remained challenging because of endothelial resistance to DNA-based gene transfer and expression. To overcome these challenges, we developed an RNA transfection method to study ET-1 posttranscriptional regulation. Reporter transcripts transfected into either preconfluent or postconfluent primary endothelial cells were rapidly and robustly expressed. RNA transfection reconstituted poly(A)-tail-dependent protein expression and ET-1 3'-UTR-dependent mRNA destabilization, suggesting that the transfected RNA accessed endothelial cell posttranscriptional pathways. Because RNA transfection uncouples transcription from expression, the influence of the ET-1 3'-UTR on posttranscriptional expression kinetics could also be monitored. Taken together, our results suggest that RNA transfection is a versatile tool to investigate ET-1 posttranscriptional regulation in endothelial cell culture models.
机译:内皮素-1(ET-1)是一种有效的内皮来源的血管收缩剂和细胞有丝分裂原。在许多心血管疾病和肾脏疾病中均观察到ET-1水平的扰动。稳态ET-1 mRNA表达在血管内皮中受到诱导型启动子和mRNA组成性半衰期的调节。最近的研究已经确定mRNA稳定是血管内皮细胞中ET-1诱导的病理生理相关机制。然而,由于内皮对基于DNA的基因转移和表达的抗性,有关生理相关的汇合后的初级内皮细胞单层中转录后途径的机制研究仍然具有挑战性。为了克服这些挑战,我们开发了一种RNA转染方法来研究ET-1转录后调控。转染到融合前或融合后原代内皮细胞中的记者转录物被迅速而稳定地表达。 RNA转染重建了poly(A)-tail依赖的蛋白表达和ET-1 3'-UTR依赖的mRNA失稳,表明转染的RNA进入了内皮细胞转录后通路。因为RNA转染使转录与表达脱钩,所以也可以监测ET-1 3'-UTR对转录后表达动力学的影响。综上所述,我们的研究结果表明RNA转染是研究内皮细胞培养模型中ET-1转录后调控的多功能工具。

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