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From mobility to crosstalk. A model of intracellular miRNAs motion may explain the RNAs interaction mechanism on the basis of target subcellular localization.从移动性到相互作用。细胞内微小RNA运动模型或许能基于靶标亚细胞定位来解释RNA的相互作用机制。
Math Biosci. 2016 Oct;280:50-61. doi: 10.1016/j.mbs.2016.07.012. Epub 2016 Aug 4.
2
Applying 3D-FRAP microscopy to analyse gap junction-dependent shuttling of small antisense RNAs between cardiomyocytes.应用3D-FRAP显微镜分析心肌细胞间小反义RNA的间隙连接依赖性穿梭。
J Mol Cell Cardiol. 2016 Sep;98:117-27. doi: 10.1016/j.yjmcc.2016.07.008. Epub 2016 Jul 29.
3
Gap junction mediated miRNA intercellular transfer and gene regulation: A novel mechanism for intercellular genetic communication.间隙连接介导的微小RNA细胞间转移与基因调控:一种细胞间遗传通讯的新机制。
Sci Rep. 2016 Jan 27;6:19884. doi: 10.1038/srep19884.
4
Role of connexin 43 in cardiovascular diseases.间隙连接蛋白 43 在心血管疾病中的作用。
Eur J Pharmacol. 2015 Dec 5;768:71-6. doi: 10.1016/j.ejphar.2015.10.030. Epub 2015 Oct 20.
5
Gap junctional shuttling of miRNA--A novel pathway of intercellular gene regulation and its prospects in clinical application.微小RNA的间隙连接穿梭——一种细胞间基因调控的新途径及其临床应用前景
Cell Signal. 2015 Dec;27(12):2506-14. doi: 10.1016/j.cellsig.2015.09.012. Epub 2015 Sep 21.
6
Circulating MicroRNAs: Potential and Emerging Biomarkers for Diagnosis of Cardiovascular and Cerebrovascular Diseases.循环微小RNA:用于诊断心脑血管疾病的潜在及新兴生物标志物
Biomed Res Int. 2015;2015:730535. doi: 10.1155/2015/730535. Epub 2015 May 28.
7
Connexin and pannexin signaling in gastrointestinal and liver disease.连接蛋白和泛连接蛋白信号传导在胃肠道和肝脏疾病中的作用
Transl Res. 2015 Oct;166(4):332-43. doi: 10.1016/j.trsl.2015.05.005. Epub 2015 May 16.
8
Gap junctions modulate glioma invasion by direct transfer of microRNA.缝隙连接通过微小RNA的直接转移来调节胶质瘤的侵袭。
Oncotarget. 2015 Jun 20;6(17):15566-77. doi: 10.18632/oncotarget.3904.
9
MicroRNAs in cardiovascular disease: an introduction for clinicians.心血管疾病中的微小RNA:临床医生入门指南
Heart. 2015 Jun;101(12):921-8. doi: 10.1136/heartjnl-2013-305402. Epub 2015 Mar 26.
10
Gap Junctions Enhance the Antiproliferative Effect of MicroRNA-124-3p in Glioblastoma Cells.缝隙连接增强微小RNA-124-3p在胶质母细胞瘤细胞中的抗增殖作用。
J Cell Physiol. 2015 Oct;230(10):2476-88. doi: 10.1002/jcp.24982.

利用三维荧光漂白恢复显微镜分析微小RNA的间隙连接依赖性转移

Analysis of the Gap Junction-dependent Transfer of miRNA with 3D-FRAP Microscopy.

作者信息

Lemcke Heiko, Voronina Natalia, Steinhoff Gustav, David Robert

机构信息

Reference and Translation Center for Cardiac Stem Cell Therapy (RTC); Department of Cardiac Surgery, University of Rostock; Department of Life, Light and Matter of the Interdisciplinary Faculty, University of Rostock;

Reference and Translation Center for Cardiac Stem Cell Therapy (RTC); Department of Cardiac Surgery, University of Rostock; Department of Life, Light and Matter of the Interdisciplinary Faculty, University of Rostock.

出版信息

J Vis Exp. 2017 Jun 19(124):55870. doi: 10.3791/55870.

DOI:10.3791/55870
PMID:28654065
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5608475/
Abstract

Small antisense RNAs, like miRNA and siRNA, play an important role in cellular physiology and pathology and, moreover, can be used as therapeutic agents in the treatment of several diseases. The development of new, innovative strategies for miRNA/siRNA therapy is based on an extensive knowledge of the underlying mechanisms. Recent data suggest that small RNAs are exchanged between cells in a gap junction-dependent manner, thereby inducing gene regulatory effects in the recipient cell. Molecular biological techniques and flow cytometric analysis are commonly used to study the intercellular exchange of miRNA. However, these methods do not provide high temporal resolution, which is necessary when studying the gap junctional flux of molecules. Therefore, to investigate the impact of miRNA/siRNA as intercellular signaling molecules, novel tools are needed that will allow for the analysis of these small RNAs at the cellular level. The present protocol describes the application of three-dimensional fluorescence recovery after photobleaching (3D-FRAP) microscopy to elucidating the gap junction-dependent exchange of miRNA molecules between cardiac cells. Importantly, this straightforward and non-invasive live-cell imaging approach allows for the visualization and quantification of the gap junctional shuttling of fluorescently labeled small RNAs in real time, with high spatio-temporal resolution. The data obtained by 3D-FRAP confirm a novel pathway of intercellular gene regulation, where small RNAs act as signaling molecules within the intercellular network.

摘要

微小反义RNA,如微小RNA(miRNA)和小干扰RNA(siRNA),在细胞生理和病理过程中发挥着重要作用,此外,还可作为治疗多种疾病的治疗剂。miRNA/siRNA治疗新的创新策略的开发基于对其潜在机制的广泛了解。最近的数据表明,小RNA以间隙连接依赖的方式在细胞间交换,从而在受体细胞中诱导基因调控效应。分子生物学技术和流式细胞术分析常用于研究miRNA的细胞间交换。然而,这些方法无法提供高时间分辨率,而这在研究分子的间隙连接通量时是必需的。因此,为了研究miRNA/siRNA作为细胞间信号分子的影响,需要新的工具来在细胞水平分析这些小RNA。本方案描述了三维光漂白后荧光恢复(3D-FRAP)显微镜在阐明心肌细胞间miRNA分子间隙连接依赖交换中的应用。重要的是,这种直接且非侵入性的活细胞成像方法能够实时可视化并定量荧光标记小RNA的间隙连接穿梭,具有高时空分辨率。通过3D-FRAP获得的数据证实了一种新的细胞间基因调控途径,即小RNA在细胞间网络中作为信号分子发挥作用。