AI Article Synopsis

  • Correlative Light Electron Microscopy (CLEM) combines light and electron microscopy techniques to address biological questions while aiming for simplicity in experimental workflows.
  • The study focuses on a straightforward CLEM approach using gridded finder imaging dishes to locate fluorescently tagged molecules in 2D cell cultures.
  • The workflow involves initial fluorescence localization via light microscopy, followed by precise localization using transmission electron microscopy (TEM), with emphasis on sample preparation steps after resin embedding.

Article Abstract

Correlative Light Electron Microscopy (CLEM) encompasses a wide range of experimental approaches with different degrees of complexity and technical challenges where the attributes of both light and electron microscopy are combined in a single experiment. Although the biological question always determines what technology is the most appropriate, we generally set out to apply the simplest workflow possible. For 2D cell cultures expressing fluorescently tagged molecules, we report on a simple and very powerful CLEM approach by using gridded finder imaging dishes. We first determine the gross localization of the fluorescence using light microscopy and subsequently we retrace the origin/localization of the fluorescence by projecting it onto the ultrastructural reference space obtained by transmission electron microscopy (TEM). Here we describe this workflow and highlight some basic principles of the sample preparation for such a simple CLEM experiment. We will specifically focus on the steps following the resin embedding for TEM and the introduction of the sample in the electron microscope.

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Source
http://dx.doi.org/10.1016/bs.mcb.2024.02.032DOI Listing

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