Literature DB >> 17406335

An ultrastructural readout of fluorescence recovery after photobleaching using correlative light and electron microscopy.

Kevin J Darcy1, Kevin Staras, Lucy M Collinson, Yukiko Goda.   

Abstract

Fluorescence recovery after photobleaching (FRAP) provides an important quantitative readout of the mobility of fluorescently tagged structures in live tissue. Here we present a protocol for visualizing FRAP signal at the ultrastructural level, permitting the nature of recovered fluorescence signal to be studied at greater resolution than afforded by conventional light microscopy. Specifically we use FRAP, fixation, photoconversion and correlative light and electron microscopy (CLEM) to examine the ultrastructural organization of mobile FM1-43-labeled vesicles in synapses of cultured hippocampal neurons. At photobleached synapses, the FRAP signal can be visualized as photoconverted electron-dense vesicles. The combination of FRAP and CLEM provides a powerful tool for examining the specific localization of imported vesicles in relation to synaptic architecture. Moreover, with the increasing availability of photoconvertible fluorophores, this approach should be readily applicable to other systems where an ultrastructural characterization of FRAP signal is desirable. After cultures are prepared and ready to use, this protocol takes 2-3 days.

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Year:  2006        PMID: 17406335     DOI: 10.1038/nprot.2006.146

Source DB:  PubMed          Journal:  Nat Protoc        ISSN: 1750-2799            Impact factor:   13.491


  18 in total

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5.  A vesicle superpool spans multiple presynaptic terminals in hippocampal neurons.

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7.  Synapsin selectively controls the mobility of resting pool vesicles at hippocampal terminals.

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8.  Extrasynaptic vesicle recycling in mature hippocampal neurons.

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10.  Single electrode dynamic clamp with StdpC.

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