Imaging of estrogen receptor-α in rat pial arterioles using a digital immunofluorescent microscope.

JOVE-JOURNAL OF VISUALIZED EXPERIMENTS(2011)

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摘要
Many of estrogen's effects on vascular reactivity are mediated through interaction with estrogen receptors 1, 2, 3. Although two sub-types exist (estrogen receptor -alpha and beta), estrogen receptor-a has been identified in both the smooth muscle and in endothelial cells of pial arterial segments using fluorescent staining combined with confocal laser scanning microscopy(4). Furthermore, ER-alpha is located in the nuclei and in the cytoplasm of rat basilar arteries(5). The receptors are abundant and fluoresce brightly, but clear visualization of discrete groups of receptors is difficult likely due to the numbers located in many cell layers of pial vessel segments. Additionally, many reports using immunohistochemical techniques paired with confocal microscopy poorly detail the requirements critical for reproduction of experiments(6). Our purpose for this article is to describe a simple technique to optimize the staining and visualization of ER-alpha using cross-sectional slices of pial arterioles obtain from female rat brains. We first perfuse rats with Evans blue dye to easily identify surface pial arteries which we isolate under a dissecting microscope. Use of a cryostat to slice 8 mu m cross sections of the arteries allows us to obtain thin vessel sections so that different vessel planes are more clearly visualized. Cutting across the vessel rather than use of a small vessel segment has the advantage of easier viewing of the endothelial and smooth muscle layers. In addition, use of a digital immunofluorescent microscope with extended depth software produces clear images of ten to twelve different vessel planes and is less costly than use of a confocal laser scanning microscope.
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Molecular Biology,Issue 57,digital immunofluorescent microscopy,brain,estrogen receptor-alpha,cerebral microvasculature,rat,immunohistochemistry
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