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a new method for evaluation of
myocardial energy metabolism
Institute of Experimental Surgery, Heinrich Heine University, 40225 Düsseldorf; and Institute of Geology, Ruhr University Bochum, 44801 Bochum, Germany
Received 10 September 1995; accepted in final form 14 June 1996.
Schwanke, Uwe, Harald Strauss, Gunther Arnold, and Jochen D. Schipke. Analysis of respiratory water
a new method for evaluation of myocardial energy metabolism. J. Appl.
Physiol. 81(5): 2115-2122, 1996.
Aerobic ATP
synthesis via oxidative phosphorylation causes a proportional
production of respiratory water. Thus the amount of respiratory water
produced at a given time should be a reliable measure of the current
ATP demand of the mammalian myocardium. Respiratory water from isolated
rabbit hearts was labeled by using the stable oxygen isotope
18O. The hearts were perfused
according to the method of Langendorff (O. Langendorff.
Pfluegers Arch. 61: 291-332,
1895) with
18O2-equilibrated
Krebs-Henseleit solution. Control hearts were exclusively perfused with
carbogen-equilibrated Krebs-Henseleit solution. Myocardial tissue was
then lyophilized; the extracted water and samples from the coronary
venous effluent were converted to
CO2 by using the guanidine
hydrochloride technique. The
18O values within the
CO2 samples were determined by
mass spectrometry and related to the standard mean ocean water
(SMOW) scale. Compared with control
hearts, the 18O-labeled hearts
exhibited a significant increase of
18O values from tissue water
(
47.50 ± 0.64 vs.
40.35 ± 2.05
SMOW; P < 0.05). The values were also
significantly increased in the coronary venous effluent after a
perfusion time of only 50 s (
47.50 ± 0.64 vs.
43.66 ± 0.91
SMOW;
P < 0.05). Thus this first
adaptation of the guanidine hydrochloride technique on microliter
samples of myocardial tissue water and coronary venous effluent
demonstrates that this method can be used to evaluate both respiratory
activity and the kinetics of cardiac metabolic processes.
isolated rabbit hearts; myocardial energy metabolism; stable oxygen isotope 18O; guanidine hydrochloride technique; mass spectrometry
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