Literature DB >> 20051381

Two-color fluorescence labeling in acrolein-fixed brain tissue.

Esther Luquin1, Eva Pérez-Lorenzo, María S Aymerich, Elisa Mengual.   

Abstract

Acrolein is a potent fixative that provides both excellent preservation of ultrastructural morphology and retention of antigenicity, thus it is frequently used for immunocytochemical detection of antigens at the electron microscopic level. However, acrolein is not commonly used for fluorescence microscopy because of concerns about possible autofluorescence and destruction of the luminosity of fluorescent dyes. Here we describe a simple protocol that allows fine visualization of two fluorescent markers in 40-mum sections from acrolein-perfused rat brain. Autofluorescence was removed by pretreatment with 1% sodium borohydride for 30 min, and subsequent incubation in a 50% ethanol solution containing 0.3% hydrogen peroxide enhanced fluorescence labeling. Thus, fluorescence labeling can be used for high-quality detection of markers in tissue perfused with acrolein. Furthermore, adjacent acrolein-fixed sections from a single experiment can be processed to produce high-quality results for electron microscopy or fluorescence labeling.

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Year:  2010        PMID: 20051381      PMCID: PMC2842598          DOI: 10.1369/jhc.2009.954495

Source DB:  PubMed          Journal:  J Histochem Cytochem        ISSN: 0022-1554            Impact factor:   2.479


  44 in total

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9.  Reduction of background autofluorescence in brain sections following immersion in sodium borohydride.

Authors:  B Clancy; L J Cauller
Journal:  J Neurosci Methods       Date:  1998-09-01       Impact factor: 2.390

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Authors:  D D SABATINI; K BENSCH; R J BARRNETT
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