Citations to this article
Abstract
Molybdenum cofactor deficiency is a devastating disease with affected patients displaying the symptoms of a combined deficiency of sulfite oxidase and xanthine dehydrogenase. Because of the extreme lability of the isolated, functional molybdenum cofactor, direct cofactor replacement therapy is not feasible, and a search for stable biosynthetic intermediates was undertaken. From studies of cocultured fibroblasts from affected individuals, two complementation groups were identified. Coculture of group A and group B cells, without heterokaryon formation, led to the appearance of active sulfite oxidase. Use of conditioned media indicated that a relatively stable, diffusible precursor produced by group B cells could be used to repair sulfite oxidase in group A recipient cells. Although the extremely low levels of precursor produced by group B cells preclude its direct characterization, studies with a heterologous, in vitro reconstitution system suggest that the precursor that accumulates in group B cells is the same as a molybdopterin precursor identified in the Neurospora crassa molybdopterin mutant nit-1, and that a converting enzyme is present in group A cells which catalyzes an activation reaction analogous to that of a converting enzyme identified in the Escherichia coli molybdopterin mutant ChlA1.
Authors
J L Johnson, M M Wuebbens, R Mandell, V E Shih
Total citations by year
Citations to this article in year 2013 (2)
| Title and authors | Publication | Year |
|---|---|---|
|
Molybdenum cofactor: A key component of Mycobacterium tuberculosis pathogenesis?
M Williams, V Mizrahi, BD Kana |
Critical Reviews in Microbiology | 2013 |
|
Metabolic stroke in a late-onset form of isolated sulfite oxidase deficiency
MD Rizzo, AP Burlina, JO Sass, F Beermann, C Zanco, C Cazzorla, A Bordugo, L Giordano, R Manara, AB Burlina |
Molecular Genetics and Metabolism | 2013 |
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