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Lady Davis Institute for Medical Research, Jewish General Hospital, Montreal, H3T 1E2; and School of Dietetics and Human Nutrition, McGill University, Sainte Anne de Bellevue, Quebec, Canada H9X 3V9
Six normal men consumed a mixed test
meal while adapted to high (1.5 g · kg
1 · day
1) and low
(0.3 g · kg
1 · day
1)
protein intakes. They completed this protocol twice: when the test
meals included 3 mg/kg of [15N]alanine
([15N]Ala) and when they included 30 mg/kg of
intrinsically labeled [15N]Spirulina platensis
([15N]SPI). Six subjects with insulin-dependent diabetes
mellitus (IDDM) receiving conventional insulin therapy consumed the
test meal with added [15N]Ala while adapted to their
customary high-protein diet. Protein restriction increased serum
alanine, glycine, glutamine, and methionine concentrations and reduced
those of leucine. Whether the previous diet was high or low in protein,
there was a similar increase in serum alanine, methionine, and
branched-chain amino acid concentrations after the test meal and a
similar pattern of 15N enrichment in serum amino acids for
a given tracer. When [15N]Ala was included in the test
meal, 15N appeared rapidly in serum alanine and glutamine,
to a minor degree in leucine and isoleucine, and not at all in other
circulating amino acids. With [15N]SPI, there was a slow
appearance of the label in all serum amino acids analyzed. Despite the
different serum amino acid labeling, protein restriction reduced the
postmeal transfer of dietary 15N in [15N]Ala
or [15N]SPI into [15N]urea by similar
amounts (38 and 43%, respectively, not significant). The response of
the subjects with IDDM was similar to that of the normal subjects.
Information about adaptive reductions in dietary amino acid catabolism
obtained by adding [15N]Ala to a test meal appears to be
equivalent to that obtained using an intrinsically labeled protein tracer.
humans; stable isotope; fed state; amino acid oxidation
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