The molecular aspects and physiological significance of NADP
+-dependent
D-arabinose dehydrogenase (ARA), which is thought to function in the biosynthesis of an analog of ascorbic acid,
D-erythroascorbic acid in yeasts, were examined. A large subunit of ARA, Ara1p produced in
E. coli, was purified as a homodimer, some of which was degraded at the N-terminus. It showed sufficient ARA activity. Degradation of Ara1p occurs naturally in yeast cells, and the small subunit of ARA previously thought as is, in fact, a naturally occuring degradation product of Ara1p. A deficient mutant of
ARA1 lost almost all NADP
+-ARA activity, but intracellular
D-erythroascorbic acid was only halved. This mutant showed increased susceptibility to H
2O
2 and diamide but not to menadione or
tert-butylhydroperoxide. Feeding
D-arabinose to mutant cells led to increases in intracellular
D-erythroascorbic acid, suggesting the presence of another ARA isozyme. The deficient mutant of
ARA1 recovered resistance to H
2O
2 with feeding of
D-arabinose. Our results suggest that the direct contributions of Ara1p both to
D-erythroascorbic acid biosynthesis and to oxidative stress resistance are quite limited.
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