Analysis of concentration and 13C enrichment of D-galactose in human plasma

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Abstract

Background: A stable-isotope dilution method for the sensitive determination of D-galactose in human plasma was established. Methods: D- [13C]Galactose was added to plasma, and the concentration was measured after D-glucose was removed from the plasma by treatment with D-glucose oxidase and the sample was purified by ion-exchange chromatography. For gas chromatographic-mass spectrometric analysis, aldononitrile pentaacetate derivatives were prepared. Monitoring of the [MH-60]+ ion intensities at m/z 328, 329, and 334 in the positive chemical ionization mode allowed the assessment of 1-12C-, 1-13C-, and U-13C6-labeled D-galactose, respectively. The D-galactose concentration was quantified on the basis of the 13C-labeled internal standard. Results: The method was linear (range examined, 0.1-5 μmol/L) and of good repeatability in the low and high concentration ranges (within- and between-run CVs <15%). The limit of quantification for plasma D-galactose was <0.02 μmol/L. Measurements in plasma of postabsorptive subjects yielded D-galactose concentrations (mean ± SD) of 0.12 ± 0.03 (n = 16), 0.11 ± 0.04 (n = 15), 1.44 ± 0.54 (n = 10), and 0.17 ± 0.07 (n = 5) μmol/L in healthy adults, diabetic patients, patients with classical galactosemia, and obligate heterozygous parents thereof, respectively. These data were considerably lower (3- to 18-fold) than the values of a conventional enzymatic assay. The procedure was also applied successfully in a stable-isotope turnover study to evaluate endogenous D-galactose formation. Conclusions: The present findings establish that detection of D-galactose from endogenous sources is feasible in human plasma and show that erroneously high results may be obtained by enzymatic methods. (C) 2000 American Association for Clinical Chemistry.

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Schadewaldt, P., Hammen, H. W., Loganathan, K., Bodner-Leidecker, A., & Wendel, U. (2000). Analysis of concentration and 13C enrichment of D-galactose in human plasma. Clinical Chemistry, 46(5), 612–619. https://doi.org/10.1093/clinchem/46.5.612

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