MicroRNA-1 prevents high-fat diet-induced endothelial permeability in apoE knock-out mice

被引:5
|
作者
Hua Wang
Hua-Qing Zhu
Feng Wang
Qing Zhou
Shu-Yu Gui
Yuan Wang
机构
[1] Anhui Medical University,Laboratory of Molecular Biology and Department of Biochemistry
[2] The Affiliated Provincial Hospital of Anhui Medical University,Department of Oncology
[3] The First Affiliated Hospital of Anhui Medical University,Department of Respiratory Disease
[4] Key Laboratory of Gene Research of Anhui Province,undefined
来源
关键词
MicroRNA-1; Permeability; Myosin light chain kinase;
D O I
暂无
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学科分类号
摘要
The development of atherosclerosis (AS) is a multifactorial process in which elevated plasma cholesterol levels play a central role. As a new class of players involved in AS, the regulation and function of microRNAs (miR) in response to AS remain poorly understood. This study analyzed the effects of miR-1 (antagomir and mimic) on endothelial permeability and myosin light chain kinase (MLCK) expression and activity in the artery wall of apoE knock-out mice after feeding them a high-cholesterol diet. Further, we tested to determine whether that effects are involved in ERK phosphorylation. Here, we show that a high-cholesterol diet induces a significant decrease of miR-1 expression. Histopathologic examination demonstrated that miR-1 antagomir enhances endothelial permeability induced by high cholesterol and miR-1 mimic attenuated endothelial barrier dysfunction. Consistent with endothelial permeability, Western blotting, qPCR, and γ-32P-ATP phosphate incorporation showed that MLCK expression and activity were further increased in miR-1 antagomir-treated mice and decreased in miR-1 mimic-treated mice compared with those of mice receiving control miR. Further mechanistic studies showed that high-cholesterol-induced extracellular signal regulated kinase (ERK) activation was enhanced by miR-1 antagomir and attenuated by miR-1 mimic. Collectively, those results indicate that miR-1 contributes to endothelial barrier function via mechanisms involving not only MLCK expression and activity but also ERK phosphorylation.
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页码:153 / 159
页数:6
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