Profiling at mRNA, protein, and metabolite levels reveals alterations in renal amino acid handling and glutathione metabolism in kidney tissue of Pept2-/- mice

Profiling at mRNA, protein, and metabolite levels reveals alterations in renal amino acid handling and glutathione metabolism in kidney tissue of Pept2-/- mice

1 Molecular Nutrition Unit, Technical University of Munich, Freising 2 Institute of Experimental Genetics, GSF, Neuherberg, Germany 3 Applied Mathematics and Informatics Unit INAPG/ENGREF/INRA, Paris, France 4 University of California Davis Genome Center, Davis, California 5 Laboratory of Bioanalysi...

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Veröffentlicht in:Physiological genomics 2007-02, Vol.28 (3), p.301-310
Hauptverfasser: Frey, Isabelle M, Rubio-Aliaga, Isabel, Siewert, Anne, Sailer, Daniela, Drobyshev, Aleksey, Beckers, Johannes, de Angelis, Martin Hrabe, Aubert, Julie, Hen, Avner Bar, Fiehn, Oliver, Eichinger, Hans M, Daniel, Hannelore
Format: Artikel
Sprache:eng
Schlagworte:
Amino Acids - metabolism
Amino Acids - urine
Animals
Dipeptides - metabolism
Dipeptides - urine
Electrophoresis, Gel, Two-Dimensional
Gene Expression Profiling
Glutathione - metabolism
Glutathione - urine
Kidney - metabolism
Mice
Mice, Inbred C57BL
Mice, Knockout
Models, Biological
Oligonucleotide Array Sequence Analysis
Proteomics
RNA, Messenger - metabolism
Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization
Symporters - genetics
Symporters - physiology
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Zusammenfassung:1 Molecular Nutrition Unit, Technical University of Munich, Freising 2 Institute of Experimental Genetics, GSF, Neuherberg, Germany 3 Applied Mathematics and Informatics Unit INAPG/ENGREF/INRA, Paris, France 4 University of California Davis Genome Center, Davis, California 5 Laboratory of Bioanalysis, Technical University of Munich, Freising, Germany PEPT2 is an integral membrane protein in the apical membrane of renal epithelial cells that operates as a rheogenic transporter for di- and tripeptides and structurally related drugs. Its prime role is thought to be the reabsorption of filtered di- and tripeptides contributing to amino acid homeostasis. To elucidate the role of PEPT2 in renal amino acid metabolism we submitted kidney tissues of wild-type and a Pept2 –/– mouse line to a comprehensive transcriptome, proteome and metabolome profiling and analyzed urinary amino acids and dipeptides. cDNA microarray analysis identified 147 differentially expressed transcripts in transporter-deficient animals, and proteome analysis by 2D-PAGE and MALDI-TOF-MS identified 37 differentially expressed proteins. Metabolite profiling by GC-MS revealed predominantly altered concentrations of amino acids and derivatives. Urinary excretion of amino acids demonstrated increased glycine and cysteine/cystine concentrations and dipeptides in urine were assessed by amino acid analysis of urine samples before and after in vitro dipeptidase digestion. Dipeptides constituted a noticeable fraction of urinary amino acids in Pept2 –/– animals, only, and dipeptide-bound glycine and cystine were selectively increased in Pept2 –/– urine samples. These findings were confirmed by a drastically increased excretion of cysteinyl-glycine (cys-gly). Urinary loss of cys-gly together with lower concentrations of cysteine, glycine, and oxoproline in kidney tissue and altered expression of mRNA and proteins involved in glutathione (GSH) metabolism suggests that PEPT2 is predominantly a system for reabsorption of cys-gly originating from GSH break-down, thus contributing to resynthesis of GSH. PEPT2; peptide transport; glutathione metabolism; pathway analysis
ISSN:1094-8341
1531-2267
DOI:10.1152/physiolgenomics.00193.2006