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Biocell 2008
A tridimensional view of the organization of actin filaments in the central nervous system by use of fluorescent photooxidationKeywords: f-actin, phalloidin-eosin phootoxidation, 3-d reconstructions, electron tomography. Abstract: cellular and subcellular organization and distribution of actin filaments have been studied with various techniques. the use of fluorescence photo-oxidation combined with phalloidin conjugates with eosin has allowed the examination of the precise cellular and subcellular location of f-actin. correlative fluorescence light microscopy and transmission electron microscopy studies of f-actin distribution are facilitated with this method for morphological and physiological studies. because phalloidin-eosin is smaller than other markers, this method allows the analysis of the three-dimensional location of f-actin with high-resolution light microscopy, three-d serial sections reconstructions, and electron tomography. the combination of selective staining and three-dimensional reconstructions provide a valuable tool for revealing aspects of the synaptic morphology that are not available when conventional electron microscopy is used. by applying this selective staining technique and three-dimensional imaging, we uncovered the structural organization of actin in the postsynaptic densities in physiological and pathological conditions.
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