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dc.contributor.authorNieves-Cintrón, Madeline
dc.contributor.authorTajada, Sendoa
dc.contributor.authorSantana, Luis Fernando
dc.contributor.authorNavedo, Manuel F.
dc.date.accessioned2024-02-06T12:00:38Z
dc.date.available2024-02-06T12:00:38Z
dc.date.issued2018
dc.identifier.citationTotal Internal Reflection Fluorescence Microscopy in Vascular Smooth Muscle. In: Trebak, Mohamed and Earley S, ed. Signal Transduction and Smooth Muscle. CRC Press; 2018:87-103es
dc.identifier.urihttps://uvadoc.uva.es/handle/10324/65813
dc.description.abstractThis chapter provides an overview of the basic concepts behind Total Internal Reflection Fluorescence Microscopy (TIRFM), and its application to the study of the function and regulation of plasmalemmal Ca2+-permeable channels in vascular smooth muscle. TIRFM utilizes an evanescent wave to selectively excite fluorophores in regions of a sample directly adjacent to the glass coverslip-buffer interface. The principles at the heart of TIRFM are based on the laws of refraction of light and properties of the refractive media. TIRFM relies on the ability to introduce light at angles exceeding a critical angle. A particular innovative use of TIRFM has been on the recording of Ca2+ signals produced by the opening of Ca2+-permeable channels at the plasma membrane of a cell, including vascular smooth muscle cells. The quality of vascular smooth muscle cells is critical for successful recording of sparklets using TIRFM. Single vascular smooth muscle cells can be obtained by enzymatic digestion of freshly dissected arteries from different vascular beds.es
dc.format.mimetypeapplication/pdfes
dc.language.isospaes
dc.rights.accessRightsinfo:eu-repo/semantics/openAccesses
dc.titleTotal Internal Reflection Fluorescence Microscopy in Vascular Smooth Musclees
dc.typeinfo:eu-repo/semantics/bookPartes
dc.type.hasVersioninfo:eu-repo/semantics/draftes


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