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Titlebook: Calcium Signaling Protocols; David G. Lambert,Richard D. Rainbow Book 2013Latest edition Springer Science+Business Media, LLC 2013 Calcium

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neue betriebswirtschaftliche forschung (nbf)erature and 45°C. The FlexStation can be configured to read a range of plate sizes. In this chapter generic methods for assessing intracellular Ca. on the FlexStation using ratiometric dyes are described.
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https://doi.org/10.1007/978-3-642-85128-5g or damage, and that the fluorescent indicator-loaded vessels behave similarly to unloaded preparations. Importantly, these approaches are applicable to both isobaric and isometric preparations and have been also used for the study of a number of vascular beds including cerebral, mesenteric, coronary, and skeletal muscle vasculatures.
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Measurement of [Ca2+]i in Whole Cell Suspensions Using Fura-2ceptors and channels. Loading characteristics and the need for agents to retain loaded dye (e.g., probenecid) need to be determined empirically. Calibration of whole cell suspensions to convert the fluorescent signal into Ca. is simply performed using Triton-X lysis (to determine ..) and EGTA chelation (to determine ..).
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Ratiometric Ca2+ Measurements Using the FlexStation®Scanning Fluorometererature and 45°C. The FlexStation can be configured to read a range of plate sizes. In this chapter generic methods for assessing intracellular Ca. on the FlexStation using ratiometric dyes are described.
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Measurement of Changes in Endothelial and Smooth Muscle Ca2+ in Pressurized Arteriesg or damage, and that the fluorescent indicator-loaded vessels behave similarly to unloaded preparations. Importantly, these approaches are applicable to both isobaric and isometric preparations and have been also used for the study of a number of vascular beds including cerebral, mesenteric, coronary, and skeletal muscle vasculatures.
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Neue Konzepte für das Kostenmanagementbed in this volume. Whole cell suspensions are loaded with Fura-2 and then placed into a cuvette-based fluorimetric system (measuring 510 nm emission at alternating 340/340 nm excitation). Cells can be stimulated with agonists and antagonists to enable temporal response profiling and concentration–r
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Neue Konzepte für das Kostenmanagementful approach to examine cellular structure and function. Allied with the development of suitable tools, it is now possible to interrogate a wide range of structural and functional aspects on both fixed and live cells. Here we describe the basic principles underlying confocal microscopy and provide m
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neue betriebswirtschaftliche forschung (nbf) dual-wavelength fluorescent probes. The FlexStation uses a Xenon flashlamp and monochromators for both excitation and emission light to allow the use of a wide range of fluorescent indicators. The system incorporates a fluid transfer system for addition of test compounds from a source plate to the
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