Literature DB >> 17229095

Analysis of synaptic ultrastructure without fixative using high-pressure freezing and tomography.

Philippe Rostaing1, Eleonore Real, Léa Siksou, Jean-Pierre Lechaire, Thomas Boudier, Tobias M Boeckers, Frank Gertler, Eckart D Gundelfinger, Antoine Triller, Serge Marty.   

Abstract

Electron microscopy allows the analysis of synaptic ultrastructure and its modifications during learning or in pathological conditions. However, conventional electron microscopy uses aldehyde fixatives that alter the morphology of the synapse by changing osmolarity and collapsing its molecular components. We have used high-pressure freezing (HPF) to capture within a few milliseconds structural features without aldehyde fixative, and thus to provide a snapshot of living synapses. CA1 hippocampal area slices from P21 rats were frozen at -173 degrees C under high pressure to reduce crystal formation, and synapses on dendritic spines were analysed after cryosubstitution and embedding. Synaptic terminals were larger than after aldehyde fixation, and synaptic vesicles in these terminals were less densely packed. Small filaments linked the vesicles in subgroups. The postsynaptic densities (PSDs) exhibited filamentous projections extending into the spine cytoplasm. Tomographic analysis showed that these projections were connected with the spine cytoskeletal meshwork. Using immunocytochemistry, we found as expected GluR1 at the synaptic cleft and CaMKII in the PSD. Actin immunoreactivity (IR) labelled the cytoskeletal meshwork beneath the filamentous projections, but was very scarce within the PSD itself. ProSAP2/Shank3, cortactin and Ena/VASP-IRs were concentrated on the cytoplasmic face of the PSD, at the level of the PSD projections. Synaptic ultrastructure after HPF was different from that observed after aldehyde fixative. The boutons were larger, and filamentous components were preserved. Particularly, filamentous projections were observed linking the PSD to the actin cytoskeleton. Thus, synaptic ultrastructure can be analysed under more realistic conditions following HPF.

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Year:  2006        PMID: 17229095     DOI: 10.1111/j.1460-9568.2006.05234.x

Source DB:  PubMed          Journal:  Eur J Neurosci        ISSN: 0953-816X            Impact factor:   3.386


  70 in total

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2.  Quantitative mass spectrometry measurements reveal stoichiometry of principal postsynaptic density proteins.

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3.  Structure and composition of the postsynaptic density during development.

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4.  New ways of looking at synapses.

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Review 5.  Balancing structure and function at hippocampal dendritic spines.

Authors:  Jennifer N Bourne; Kristen M Harris
Journal:  Annu Rev Neurosci       Date:  2008       Impact factor: 12.449

Review 6.  Seeing the forest tree by tree: super-resolution light microscopy meets the neurosciences.

Authors:  Marta Maglione; Stephan J Sigrist
Journal:  Nat Neurosci       Date:  2013-06-25       Impact factor: 24.884

Review 7.  Spine remodeling and synaptic modification.

Authors:  Xiao-bin Wang; Qiang Zhou
Journal:  Mol Neurobiol       Date:  2010-01-06       Impact factor: 5.590

8.  The actin-binding protein Abp1 controls dendritic spine morphology and is important for spine head and synapse formation.

Authors:  Akvile Haeckel; Rashmi Ahuja; Eckart D Gundelfinger; Britta Qualmann; Michael M Kessels
Journal:  J Neurosci       Date:  2008-10-01       Impact factor: 6.167

Review 9.  Ena/VASP: proteins at the tip of the nervous system.

Authors:  Frauke Drees; Frank B Gertler
Journal:  Curr Opin Neurobiol       Date:  2008-05-26       Impact factor: 6.627

Review 10.  Glutamate receptor dynamics in dendritic microdomains.

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