Abstract

A simple model describing reactions of alanine metabolism in isolated hepatocytes from fasted rats is proposed and applied to radioactive data obtained in experiments in which l-[1- 14C]-, l-[2- 14C]-, l-[3- 14C]-, and l-[U- 14C]alanine as well as l-alanine plus NaH 14CO 3 were used as substrates in parallel. Measurements of the rates of incorporation of the label into glucose and CO 2 and of accumulation of [1- 14C]pyruvate, [1- 14C]lactate, [1- 14C]alanine and [1- 14C]glutamate plus [1- 14C]glutamine from the different substrates used allows to calculate flux of alanine carbon through the various metabolic steps taken into account in the model. The validity of this model is indicated by the agreement found between calculations and measurement of the 14CO 2 released from [1- 14C]alanine as well as between the values of flux through pyruvate carboxylase calculated in two different ways. It is shown that the oxaloacetate synthesized by pyruvate carboxylase enters into the Krebs cycle and into the pathway of phospho enol pyruvate synthesis in about equal proportions and that about 40% of the oxaloacetate synthesized as a result of alanine metabolism is derived from the Krebs cycle operation. These results, together with the conclusion that flux of alanine carbon through pyruvate dehydrogenase is negligible, are in agreement with known characteristics of hepatic alanine metabolism in the fasted state and, therefore, provide further evidence for the validity of the model proposed in the present study.

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