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JBC, Vol. 250, Issue 15, 5866-5876, Aug, 1975
G. J. Raugi, T. Liang and J. J. Blum
A detailed model of intermediary metabolism has been constructed which is
consistent with all known information on the compartmental structure of
metabolism in Tetrahymena, on the enzyme complement of this cell, and on
the localization of the enzymes. The model allows computation of the
specific activity of every carbon atom of all metabolites and thus of the
flux of carbon along the major pathways of metabolism under steady state
conditions. To test the model, data were required from cells grown under
standard conditions and then suspended in a dilute salt solution and
incubated for 1 hour in a mixture of acetate, pyruvate, hexanoate,
bicarbonate, and glutamate labeled in a total of 10 positions, but with
only one substrate labeled in any given flask. Twenty-seven measurements of
label incorporation into CO2, lipids, glycogen, glutamate, and alanine were
made, plus measurements of label distribution into fatty acid and glycerol
moieties for 4 of the substrates and of oxygen consumption and of
glycogenolysis, yielding 33 independent measurements. These, plus about 18
"limit" measurements which also constrain any possible solutions, were in
sufficient excess of the 23 independent parameters to permit a stringent
assessment of the model. Equations derived directly from the structure of
the model and from the known stereochemistry of the reactions were
programmed on a PDP-15 computer and values of the Qo2 and of label expected
to be incorporated into the various products actually measured were
computed for any given set of flux rates. A set of flux rates was found
which yielded an excellent fit to the observed data. The ability to achieve
a fit to the data for an overdetermined system constitutes strong support
for this structural model of intermediary metabolism and the computed flux
rates therefore provide a quantitative description of metabolite flow in
the intact cell. Despite the redundancy of measurements relative to
parameters to be determined, it was not possible to define a unique set of
values for the flux through phosphoenolpyruvate carboxylase and
phosphoenolpyruvate carboxykinase, although the relationship between these
fluxes is specified by the model. The analysis allows estimation of the
recycling of phosphoenopyruvate through pyruvate kinase under conditions of
net glyconeogenesis and an apparently futile exchange of acetyl-CoA between
the inner and outer mitochondrial compartments. Carbon flow through the
glyoxylate bypass under these conditions is about one-third of that through
the Krebs cycle. The analysis also shows a net transport of malate from the
peroxisomes to the mitochondria, consistent with the anaplerotic role of
the peroxisomal glyoxylate bypass in Tetrahymena.
A quantitative analysis of metabolite fluxes along some of the pathways of intermediary metabolism in Tetrahymena pyriformis
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