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      The neurotransmitter receptor-anchoring protein gephyrin reconstitutes molybdenum cofactor biosynthesis in bacteria, plants, and mammalian cells.

      Proceedings of the National Academy of Sciences of the United States of America
      Animals, Carrier Proteins, genetics, metabolism, Cloning, Molecular, Coenzymes, Escherichia coli, Escherichia coli Proteins, Gene Expression Regulation, L Cells (Cell Line), Mammals, Membrane Proteins, Metalloproteins, Mice, Plants, Genetically Modified, Plants, Toxic, Pteridines, Rats, Recombinant Proteins, biosynthesis, Sulfurtransferases, Tobacco, Transfection

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          Abstract

          The molybdenum cofactor (Moco), a highly conserved pterin compound complexing molybdenum, is required for the enzymatic activities of all molybdenum enzymes except nitrogenase. Moco is synthesized by a unique and evolutionarily old pathway that requires the activities of at least six gene products. Some of the proteins involved in bacterial, plant, and invertebrate Moco biosynthesis show striking homologies to the primary structure of gephyrin, a polypeptide required for the clustering of inhibitory glycine receptors in postsynaptic membranes in the rat central nervous system. Here, we show that gephyrin binds with high affinity to molybdopterin, the metabolic precursor of Moco. Furthermore, gephyrin expression can reconstitute Moco biosynthesis in Moco-deficient bacteria, a molybdenum-dependent mouse cell line, and a Moco-deficient plant mutant. Conversely, inhibition of gephyrin expression by antisense RNA expression in cultured murine cells reduces their Moco content significantly. These data indicate that in addition to clustering glycine receptors, gephyrin also is involved in Moco biosynthesis and illustrate the remarkable conservation of its function in Moco biosynthesis throughout phylogeny.

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