AJP - Heart Calcium Transients and Cell-Sarcomere
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Am J Physiol Heart Circ Physiol 287: H1801-H1812, 2004. First published May 20, 2004; doi:10.1152/ajpheart.00232.2004
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Coverslip hypoxia: a novel method for studying cardiac myocyte hypoxia and ischemia in vitro

Kelly R. Pitts and Christopher F. Toombs

Department of Inflammation Research, Amgen Incorporated, Seattle, Washington 98119-3105

Submitted 9 March 2004 ; accepted in final form 12 May 2004

In vitro experimental models designed to study the effects of hypoxia and ischemia typically employ oxygen-depleted media and/or hypoxic chambers. These approaches, however, allow for metabolites to diffuse away into a large volume and may not replicate the high local concentrations that occur in ischemic myocardium in vivo. We describe herein a novel and simple method for creating regional hypoxic and ischemic conditions in neonatal rat cardiac myocyte monolayers. This method consists of creating a localized diffusion barrier by placing a glass coverslip over a portion of the monolayer. The coverslip restricts covered myocytes to a thin film of media while leaving uncovered myocytes free to access the surrounding bulk media volume. Myocytes under the coverslip undergo marked morphology changes over time as assessed by video microscopy. Fluorescence microscopy shows that these changes are accompanied by alterations in mitochondrial membrane potential and plasma membrane dynamics and eventually result in myocyte death. We also show that the metabolic activity of myocytes drives cell necrosis under the coverslip. In addition, the intracellular pH of synchronously contracting myocytes under the coverslip drops rapidly, which further implicates metabolic activity in regulating cell death under the coverslip. In contrast with existing models of hypoxia/ischemia, this technique provides a simple and effective way to create hypoxic/ischemic conditions in vitro. Moreover, we conclude that myocyte death is hastened by the combination of hypoxia, metabolites, and acidosis and is facilitated by a reduction in media volume, which may better represent ischemic conditions in vivo.

monolayer; diffusion barrier; necrosis; cell death; ischemia; myocyte



Address for reprint requests and other correspondence: C. F. Toombs, Amgen, Inc., 1201 Amgen Ct. West, Seattle, WA 98119-3105 (E-mail: ctoombs{at}amgen.com)




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