ausblenden:
Schlagwörter:
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Zusammenfassung:
Cryofixation yields outstanding ultrastructural preservation of cells
for electron microscopy, but current methods disrupt live cell
imaging. Here we demonstrate a microfluidic approach that
enables cryofixation to be performed directly in the light
microscope with millisecond time resolution and at atmospheric
pressure. This will provide a link between imaging/stimulation of
live cells and post-fixation optical, electron, or X-ray microscopy.