Journal of Biochemistry

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J. Biochem, 2004, Vol. 135, No. 2 225-230
© 2004 The Japanese Biochemical Society

MOLECULAR BIOLOGY

Disruption of the plr1 ⁺ Gene Encoding Pyridoxal Reductase of Schizosaccharomyces pombe

Tomotake Morita¹, Kaoru Takegawa² and Toshiharu Yagi^*,1

¹ Department of Bioresources Science, Faculty of Agriculture, Kochi University, Nankoku, Kochi 783-8502; and ² Department of Life Sciences, Faculty of Agriculture, Kagawa University, Kagawa 761-0795

Pyridoxal (PL) reductase encoded by the plr1⁺ gene practically catalyzes the irreversible reduction of PL by NADPH to form pyridoxine (PN). The enzyme has been suggested to be involved in the salvage synthesis of pyridoxal 5'-phosphate (PLP), a coenzyme form of vitamin B₆, or the excretion of PL as PN from yeast cells. In this study, a PL reductase-disrupted (plr1) strain was constructed and its phenotype was examined. The plr1 cells showed almost the same growth curve as that of wild-type cells in YNB and EMM media. In EMM, the plr1 strain became flocculent at the late stationary phase for an unknown reason. The plr1 cells showed low but measurable PL reductase activity catalyzed by some other protein(s) than the enzyme encoded by the plr1⁺ gene, which maintained the flow of "PL PN PNP PLP" in the salvage synthesis of PLP. The total vitamin B₆ and pyridoxamine 5'-phosphate contents in the plr1 cells were significantly lower than those in the wild-type ones. The percentages of the PLP amount as to the other vitamin B₆ compounds were similar in the two cell types. The amount of PL in the culture medium of the disruptant was significantly higher than that in the wild-type. In contrast, PN was much higher in the latter than the former. The plr1 cells accumulated a 6.1-fold higher amount of PL than the wild-type ones when they were incubated with PL. The results showed that PL reductase encoded by the plr1⁺ gene is involved in the excretion of PL after reducing it to PN, and may not participate in the salvage pathway for PLP synthesis.

^* To whom correspondence should be addressed. Tel/Fax: +81-88-864-5191, E-mail: yagito{at}cc.kochi-u.ac.jp

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