Literature DB >> 9343585

Dynamic imaging of purified individual synaptic vesicles.

V Parpura1, R T Doyle, T A Basarsky, E Henderson, P G Haydon.   

Abstract

The atomic force microscope (AFM) was used to directly image purified synaptic vesicles. Individual secretory vesicles (approximately 50 nm diameter) were resolved with the AFM when imaged either dry or in solution. Vesicles were observed repeatedly for periods of greater than 2 h. To ask whether the AFM can detect structural change of vesicles the osmolarity of the bathing medium was reduced from 330 to 110 mOsm. Hypo-osmotic treatment caused an expansion and flattening of the vesicles. Thus, using the AFM it is possible to resolve individual vesicles and follow changes in vesicular structure. This opens the possibility that the secretory event can be reconstituted and visualized in vitro in order to elucidate the roles of synaptic proteins in synaptic transmission.

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Year:  1995        PMID: 9343585     DOI: 10.1006/nimg.1995.1003

Source DB:  PubMed          Journal:  Neuroimage        ISSN: 1053-8119            Impact factor:   6.556


  8 in total

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4.  Atomic force microscopy study of the secretory granule lumen.

Authors:  V Parpura; J M Fernandez
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5.  Changes in the elastic properties of cholinergic synaptic vesicles as measured by atomic force microscopy.

Authors:  D E Laney; R A Garcia; S M Parsons; H G Hansma
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Journal:  Hum Mol Genet       Date:  2011-01-21       Impact factor: 6.150

7.  Formation of cholesterol crystals at a mucin coated substrate.

Authors:  Xiangmin Liao; Timothy S Wiedmann
Journal:  Pharm Res       Date:  2006-08-23       Impact factor: 4.200

8.  Influence of synapsin I on synaptic vesicles: an analysis by force-volume mode of the atomic force microscope and dynamic light scattering.

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Journal:  Biophys J       Date:  2007-05-04       Impact factor: 4.033

  8 in total

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