Encyclopedia of Experiments
Recherche en cancérologie
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Encyclopedia of Experiments Recherche en cancérologie
Cerebellum Dissection and Slice Preparation: A Method to Generate Tissue Slices from Mouse Cerebellum

Cerebellum Dissection and Slice Preparation: A Method to Generate Tissue Slices from Mouse Cerebellum

Transcription

To begin, insert a small scissors gently into the foramen magnum and cut the skull by making one lateral incision towards the side and then cut all around the head skull. To retrieve the dorsal part of the skull, use a fine straight forceps to carefully lift the dorsal part of the skull.

Then, carefully introduce the forceps between the ventral skull and the brain. Gently flip out the brain and cut the optic and trigeminal nerves with small scissors. Next, turn the head or the dorsal part of the skull upside down just above a 60-millimeter cell culture dish containing ice-cold dissection medium to help the brain to drop by gravity.

Using fine forceps, orientate the brain with the dorsal side facing up and the ventral side lying down. Under the binocular microscope, use the fine straight forceps to immobilize the brain on the forebrain side. Then, separate the hindbrain from the rest of the brain. Cut the cerebellar peduncles underneath the cerebellum to separate the cerebellum from the rest of the hindbrain.

Once the cerebellum is isolated, use fine straight forceps to carefully tear away the meninges. Hold the cerebellum gently with the fine curved forceps and place it with the dorsal side up onto the plastic platform perpendicular to the chopper razor blade. Next, with a sterile thin end pipette tip attached to a 1-milliliter pipette, aspirate any excess of dissection medium around the cerebellum. Then, with a tissue chopper sliced 300-micrometer thick sagittal sections of the cerebellum.

Next, add a drop of dissection medium onto the sliced cerebellum gently. Then, with a wide-bore pipette tip attached to the 1-milliliter pipette, slowly aspirate the sliced cerebellum and transfer it back into the 60-millimeter cell culture dish containing ice-cold dissection medium.

Next, use two fine straight forceps to separate individual slices. Then, with a wide-bore pipette tip attached to the 1-milliliter pipette, transfer up to four selected slices from the vermis along with some dissection medium onto one culture insert of a 6-well plate. Remove any excess of dissection medium around the slices using a thin-end pipette tip.

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