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Freeze substitution of rapidly cooled human sperm.
No cryoprotectant was used. Ice was nucleated within the straw at -7°C.
The sample was then cooled at 1000°C per minute to -100°C and
then transferred to liquid nitrogen. The sample was cross fractured and
then freeze substituted. Electron microscopy shows details of sperm cells
embedded within the freeze concentrated material.
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