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J. Biol. Chem., Vol. 263, Issue 4, 1665-1675, Feb, 1988
Mechanisms of oxidant-mediated cell injury. The glycolytic and mitochondrial pathways of ADP phosphorylation are major intracellular targets inactivated by hydrogen peroxide
PA Hyslop, DB Hinshaw, WA Halsey Jr, IU Schraufstatter, RD Sauerheber, RG Spragg, JH Jackson and CG Cochrane
Department of Immunology, Scripps Clinic and Research Foundation, La Jolla, California 92037.
Inhibition of ADP phosphorylation by both glycolysis and mitochondria in
P388D1 cells exposed to H2O2 is described. Net glucose uptake and lactate
production were inhibited by oxidant exposure (ED50 = 50-100 microM).
Glycolysis was specifically inactivated at the glyceraldehyde- 3-phosphate
dehydrogenase step by three independent mechanisms: (a) direct inactivation
of the intracellular enzyme (ED50 approximately equal to 100 microM); (b)
reduction of the intracellular concentration and redox potential of its
nicotinamide cofactors; and (c) a cytosolic pH shift further from the
enzyme optima. Consistent with inhibition of glycolysis at the
glyceraldehyde-3-phosphate dehydrogenase step, a rise in the intracellular
concentration of glyceraldehyde 3-phosphate, dihydroxyacetone phosphate,
and fructose 1,6-bisphosphate was observed. The calculated combined
inhibition of glyceraldehyde-3-phosphate dehydrogenase activity could be
reasonably correlated with the depression in glycolytic flux rate with the
appropriate modeling. The steady-state contribution by mitochondria to the
total intracellular ATP pool was indirectly determined by the use of
various metabolic inhibitors and was found to rapidly decline following
exposure to 300- 800 microM H2O2. The inhibition of ADP phosphorylation
appeared to be related more to the direct inhibition of the ATPase-synthase
complex rather than to the diminished capacity of the respiratory chain for
coupled electron transport. Both the estimated rates of ADP phosphorylation
by glycolysis and mitochondria and the estimated rate of ATP hydrolysis by
ongoing metabolism were utilized to model the approximate decline in
intracellular ATP expected at 15-min exposure to various H2O2
concentrations. Theoretical calculations and the measured intracellular ATP
status were in good agreement. Oxidant exposure for 15 min resulted in
dose-dependent killing of the cells (ED50 = 500 microM), indicating a close
correlation between H2O2-mediated loss of intracellular ATP and cell
viability. The possible contribution of impaired energy homeostasis during
oxidant-mediated injury to the process of cell dysfunction and death is
discussed.

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Copyright © 1988 by the American Society for Biochemistry and Molecular Biology.
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