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01507nam a2200265Ia 4500 |
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10-1016-j-xpro-2022-101301 |
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220425s2022 CNT 000 0 und d |
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|a 26661667 (ISSN)
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|a Protocol to record and quantify the intracellular pH in contracting cardiomyocytes
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|b Cell Press
|c 2022
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|z View Fulltext in Publisher
|u https://doi.org/10.1016/j.xpro.2022.101301
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|a Intracellular pH (pHi) plays critical roles in the regulation of cardiac function. Methods and techniques for cardiac pHi measurement have continued to evolve since early 1960s. Fluorescent microscopy is the most recently developed technique with several advantages over other techniques including higher spatial and temporal resolutions, and feasibility for contracting cell measurement. Here, we describe detailed methods for mouse cardiomyocyte isolation, and simultaneous measurement and quantification of pHi and sarcomere length in contracting cardiomyocytes. For complete details on the use and execution of this protocol, please refer to Lyu et al. (2022). © 2022 The Author(s)
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|a Cell isolation
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|a Cell-based Assays
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|a Metabolism
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|a Microscopy
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|a Single Cell
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|a Chiamvimonvat, N.
|e author
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|a Lyu, Y.
|e author
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|a Overton, J.
|e author
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|a Thai, P.N.
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|a Timofeyev, V.
|e author
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|a Yamoah, E.N.
|e author
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|a Zhang, X.-D.
|e author
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|t STAR Protocols
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