Bu içeriği görüntülemek için JoVE aboneliği gereklidir.
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Begin with an anesthetized mouse with a headplate secured over a surgically prepared thin-skull cortical window.
Position the mouse supine. Remove the medial thigh skin to expose the femoral vein.
Inject a fluorescent dye conjugate into the vein to label blood plasma, enabling blood vessel visualization.
Suture the incision.
Flip the mouse and secure the headplate in a harness to stabilize the mouse.
Transfer the setup to a two-photon microscope stage.
Add saline over the cortical window. Lower the objective lens until it contacts the saline.
Using bright-field illumination, locate the imaging region.
Switch to two-photon imaging.
The microscope’s laser focuses low-energy near-infrared light into the brain.
At the laser’s focal point, two photons combine their energy to excite the dye, making the blood vessels fluoresce.
Identify a capillary bed—a network of small blood vessels connecting arteries to veins— and magnify it.
Acquire images to analyze the brain’s microvasculature.
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