Production of 1-Carbon Units from Glycine Is Extensive in Healthy Men and Women

Lamers, Yvonne; Williamson, Jerry; Theriaque, Douglas W.; Shuster, Jonathan J.; Gilbert, Lesa R.; Keeling, Christine; Stacpoole, Peter W.; Gregory, Jesse F.

doi:10.3945/jn.108.103580

Cited by 32 publications

(29 citation statements)

References 25 publications

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“…We did not detect the enrichment of either glycolate or oxalate with a single labeled carbon, indicating that the metabolism did not involve the splitting of the carbon-carbon bond. Whole body flux values were calculated for each of the glycine infusion levels (Table 2) and were similar to those previously reported [23][24][25][26][27]. Our results suggest that glycine metabolism increased at the higher infusion rate when plasma glycine levels were increased, as the flux was 72% higher (P = 0.02).…”

Section: Infusion With [12-13 C 2 ] Glycine At 60 µMoles/kg/hrsupporting

confidence: 70%

2061 Metabolism of Primed, Constant Infusions of [1,2-13c2] Glycine and [1-13c1] Phenylalanine to Urinary Oxalate

et al. 2011

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Objective-Experiments in humans and rodents using oral doses of glycine and phenylalanine have suggested that the metabolism of these amino acids contributes to urinary oxalate excretion. To better define this contribution we have examined the primed, constant infusion of [1-13 C 1 ] phenylalanine and [1,2-13 C 2 ] glycine in the post-absorptive state in healthy adults.Materials/Methods-Subjects were infused for 5 hours, collected hourly urines and had blood drawn every 30 minutes. Ion chromatography/mass spectrometry was used to measure [ 13 C] enrichment in urinary oxalate, glycolate and hippurate, and the enrichment of 13 C-amino acids in plasma samples was measured by gas chromatography/mass spectrometry.Results-Following infusion with either 6 µmoles/kg/hr [1-13 C 1 ] phenylalanine or 6 µmoles/kg/ hr [1,2-13 C 2 ] glycine, no isotopic glycolate or oxalate was detected in urine. Based on the limits of detection of our ion chromatography/mass spectroscopy method, these data indicate that < 0.7% of the urinary oxalate could be derived from phenylalanine catabolism and < 5% from glycine catabolism. Infusions with high levels of [1,2-13 C 2 ] glycine, 60 µmoles/kg/hr, increased mean plasma glycine by 29% and the whole body flux of glycine by 72%. Under these conditions glycine contributed 16.0 ± 1.6% and 16.6 ± 3.2% to urinary oxalate and glycolate excretion, respectively. Experiments using cultured hepatoma cells demonstrated that only at supraphysiological levels (>1mM) did glycine and phenylalanine metabolism increase oxalate synthesis.Conclusions-These data suggest glycine and phenylalanine metabolism make only minor contributions to oxalate synthesis and urinary oxalate excretion.

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Section: Infusion With [12-13 C 2 ] Glycine At 60 µMoles/kg/hrsupporting

confidence: 70%

2061 Metabolism of Primed, Constant Infusions of [1,2-13c2] Glycine and [1-13c1] Phenylalanine to Urinary Oxalate

et al. 2011

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“…see Refs. [1][2][3][4][5][6]. Because the GCS-catalyzed reactions are reversible (7,8), they can also perform de novo synthesis of glycine from one-carbon units, CO 2 , and NH 3 (9,10).…”

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confidence: 99%

Structure of the Homodimeric Glycine Decarboxylase P-protein from Synechocystis sp. PCC 6803 Suggests a Mechanism for Redox Regulation

Hasse

Andersson

Carlsson

et al. 2013

Journal of Biological Chemistry

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Background: Glycine decarboxylase (P-protein) is essential for many vital processes, including nucleotide biosynthesis and photosynthesis. Results: Disulfide formation drives conformational changes that inactivate the cyanobacterial P-protein, a model for plant and human glycine decarboxylase. Conclusion: Glycine decarboxylase activity is regulated by cellular redox homeostasis. Significance: This is the first molecular model for redox regulation of glycine decarboxylase.

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“…However, a recent metabolomics study indicates that cytosolic purine synthesis incorporate carbon 13-labeled glycine only by direct incorporation by the glycinamide ribonucleotide synthetase reaction and not by 1-carbon transfers of C2 and C8 of the purine ring, and that the majority of C5-methyl groups of thymidylate come from serine and not mitochondrial glycine (37). Studies in intact mouse embryos and whole body studies in humans suggest that the majority of the methyl groups donated to S-adenosylhomocysteine are derived from mitochondrial folate metabolism and that the mitochondrial GCS generates as much as 20 times more 1-carbon units than needed for all methylation reactions (38,39). Recent studies have broadened our perspectives on mitochondrial 1-carbon metabolism with the observation that the large percentage of mitochondrial glycine-derived 1-carbon units in mammalian-transformed cells are oxidized completely, generating a major proportion of cellular NADPH (37).…”

Section: Discussionmentioning

confidence: 99%

Mammalian Mitochondrial and Cytosolic Folylpolyglutamate Synthetase Maintain the Subcellular Compartmentalization of Folates

Lawrence

Titus

Ferguson

et al. 2014

Journal of Biological Chemistry

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Background: Folylpolyglutamates are in the cytosol and mitochondria and the enzyme that makes these compounds, folylpolyglutamate synthetase (FPGS) is in both compartments. Results: Folylpolyglutamates cannot traverse mitochondrial membranes in either direction. Conclusion: Subcellular isoforms of FPGS are required to establish and maintain subcellular folate compartmentalization and function. Significance: Mitochondrial folates are a separate metabolic pool not in equilibrium with cytosol.

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Production of 1-Carbon Units from Glycine Is Extensive in Healthy Men and Women

Cited by 32 publications

References 25 publications

2061 Metabolism of Primed, Constant Infusions of [1,2-13c2] Glycine and [1-13c1] Phenylalanine to Urinary Oxalate

2061 Metabolism of Primed, Constant Infusions of [1,2-13c2] Glycine and [1-13c1] Phenylalanine to Urinary Oxalate

Structure of the Homodimeric Glycine Decarboxylase P-protein from Synechocystis sp. PCC 6803 Suggests a Mechanism for Redox Regulation

Mammalian Mitochondrial and Cytosolic Folylpolyglutamate Synthetase Maintain the Subcellular Compartmentalization of Folates

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