Literature DB >> 28654065

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

Heiko Lemcke1, Natalia Voronina2, Gustav Steinhoff2, Robert David3.   

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.

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Year:  2017        PMID: 28654065      PMCID: PMC5608475          DOI: 10.3791/55870

Source DB:  PubMed          Journal:  J Vis Exp        ISSN: 1940-087X            Impact factor:   1.355


  31 in total

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Review 2.  Gap junctional shuttling of miRNA--A novel pathway of intercellular gene regulation and its prospects in clinical application.

Authors:  Heiko Lemcke; Gustav Steinhoff; Robert David
Journal:  Cell Signal       Date:  2015-09-21       Impact factor: 4.315

3.  Beyond photobleaching, laser illumination unbinds fluorescent proteins.

Authors:  Katrin G Heinze; Santiago Costantino; Paul De Koninck; Paul W Wiseman
Journal:  J Phys Chem B       Date:  2009-04-16       Impact factor: 2.991

4.  Potent and specific genetic interference by double-stranded RNA in Caenorhabditis elegans.

Authors:  A Fire; S Xu; M K Montgomery; S A Kostas; S E Driver; C C Mello
Journal:  Nature       Date:  1998-02-19       Impact factor: 49.962

5.  Endogenous RNAs modulate microRNA sorting to exosomes and transfer to acceptor cells.

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Journal:  Cell Rep       Date:  2014-08-21       Impact factor: 9.423

6.  From mobility to crosstalk. A model of intracellular miRNAs motion may explain the RNAs interaction mechanism on the basis of target subcellular localization.

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8.  Dominant connexin26 mutants associated with human hearing loss have trans-dominant effects on connexin30.

Authors:  Sabrina W Yum; Junxian Zhang; Steven S Scherer
Journal:  Neurobiol Dis       Date:  2010-01-21       Impact factor: 5.996

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Authors:  Heiko Lemcke; Marie-Louise Nittel; Dieter G Weiss; Sergei A Kuznetsov
Journal:  Eur J Neurosci       Date:  2013-04-22       Impact factor: 3.386

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Journal:  Ann N Y Acad Sci       Date:  2004-04       Impact factor: 5.691

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  2 in total

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2.  How Does a Tumor Get Its Shape? MicroRNAs Act as Morphogens at the Cancer Invasion Front.

Authors:  Catalin Vasilescu; Mihai Tanase; Dana Giza; Livia Procopiuc; Mihnea P Dragomir; And George A Calin
Journal:  Noncoding RNA       Date:  2020-06-10
  2 in total

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