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Sectioning, Staining and TEM Imaging of Embedded Exosomes: A Protocol To Visualize the Structural Features of Exosomes Using TEM

Published: April 30, 2023

Abstract

Source: Jung, M. K. et al. Sample Preparation and Imaging of Exosomes by Transmission Electron Microscopy. J. Vis. Exp. (2018)

This video describes the technique for preparing a thin section of embedded exosomes. These sections can further be stained and imaged using transmission electron microscopy, or TEM, to study the structural features of exosomes.

Protocol

1. Sectioning of the Exosomes

  1. Prepare exosome block by embedding the purified exosome sample (obtained from the culture supernatant of HCT116 cells) in pure low viscosity embedding mixture.
  2. Section the exosome block with 60 nm thickness through an ultra-microtome.
  3. Double stain with 2% uranyl acetate for 20 min and lead citrate for 10 min.
    For Reynolds lead solution, add 1.33 g of lead nitrate and 1.76 g of sodium citrate to a total of 50 mL distilled water.
  4. Observe the grid under transmission electron microscopy at 80 kV.
  5. Click "Acquire" and then click "File" and "Save as" in the CCD camera system under the electron microscope at 80 kV. Follow automatic settings for the exposure time.

Disclosures

The authors have nothing to disclose.

Materials

Ultra-microtome Leica UCT
Uranyl acetate EMS 22400 Hazardous chemical
Lead citrate EMS 17900
Transmission Electron Microscopy Hitachi H7600
Nickel grid EMS G200-Ni
Copper grid EMS G200-Cu
Transmission Electron Microscopy JEOL JEM2200FS

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Cite This Article
Sectioning, Staining and TEM Imaging of Embedded Exosomes: A Protocol To Visualize the Structural Features of Exosomes Using TEM. J. Vis. Exp. (Pending Publication), e20418, doi: (2023).

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