Em observations of microsomes
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LEVEL I
Figure 7.3 Isolated microsomes
Figure 7.4 TEM of hepatocyte
MATERIALS
- 1% Glutaraldehye (GTA)
- 1% Osmium tetroxide
- Epoxy or vinyl resin for TEM
- TEM photomicrograph of liver cells
- Transmission electron microscope
PROCEDURE
- Place a mm piece of the final pellet from Exercise 7.1 into a small vial containing 1% GTA. Fix the pellet for 2 hours.
- Rinse the pellet with water and place in three changes of water for 30 minutes each, to remove any residual GTA.
- Post fix the lysosome pellet in 1% osmium tetroxide for 1 hour. Wash thoroughly with 3 changes of water (30 minutes each).
- Dehydrate the tissue by passing through a series of graded alcohols or acetone, and embed in plastic blocks.
- Section the plastic blocks and place on coated grid. Double stain with uranyl acetate and lead nitrate and examine with a transmission electron microscope.
- Compare the view of the compacted lysosome pellet to the structure and distribution of microsomes in an intact hepatocyte (liver cell). Use figures 7.3 and 7.4 for reference.