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Abstract
Recently it was proposed that the redox status of cysteines acts as a redox switch to regulate both the oligomeric status and the activity of human dUTPase. In a separate report, a human dUTPase point mutation, resulting in a tyrosine to cysteine substitution (Y54C) was identified as the monogenic cause of a rare syndrome associated with diabetes and bone marrow failure. These issues prompt a critical investigation about the potential regulatory role of cysteines in the enzyme. Here we show on the one hand that independently of the redox status of wild-type cysteines, human dUTPase retains its characteristic trimeric assembly and its catalytic activity. On the other hand, the Y54C mutation did not compromise the substrate binding and the catalytic properties of the enzyme at room temperature. The thermal stability of the mutant protein was found to be decreased, which resulted in the loss of 67% of its activity after 90 min incubation at the physiological temperature in contrast to the wild-type enzyme. In addition, the presence or absence of reducing agents had no effect on hDUTY54C activity and stability, although it was confirmed that the introduced cysteine contains a solvent accessible thiol group.
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Details
1 RCNS, Eötvös Loránd Research Network, Institute of Enzymology, Budapest, Hungary (GRID:grid.429187.1) (ISNI:0000 0004 0635 9129); Budapest University of Technology and Economics, Department of Applied Biotechnology and Food Sciences, Budapest, Hungary (GRID:grid.6759.d) (ISNI:0000 0001 2180 0451)
2 Budapest University of Technology and Economics, Department of Applied Biotechnology and Food Sciences, Budapest, Hungary (GRID:grid.6759.d) (ISNI:0000 0001 2180 0451)
3 Semmelweis University, Department of Biochemistry, Institute of Biochemistry and Molecular Biology, Budapest, Hungary (GRID:grid.11804.3c) (ISNI:0000 0001 0942 9821)