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First published online February 13, 2003; 10.1104/pp.102.014639

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Plant Physiol, March 2003, Vol. 131, pp. 1250-1257

Enhanced Selenium Tolerance and Accumulation in Transgenic Arabidopsis Expressing a Mouse Selenocysteine Lyase1

Marinus Pilon, Jennifer D. Owen, Gulnara F. Garifullina, Tatsuo Kurihara, Hisaaki Mihara, Nobuyoshi Esaki, and Elizabeth A.H. Pilon-Smits*

Department of Biology, Colorado State University, Anatomy/Zoology Building, Fort Collins, Colorado 80523 (M.P., J.D.O., G.F.G., E.A.H.P.-S.); and Institute for Chemical Research, Kyoto University, Uji, Kyoto 611-0011, Japan (T.K., H.M., N.E.)

Selenium (Se) toxicity is thought to be due to nonspecific incorporation of selenocysteine (Se-Cys) into proteins, replacing Cys. In an attempt to direct Se flow away from incorporation into proteins, a mouse (Mus musculus) Se-Cys lyase (SL) was expressed in the cytosol or chloroplasts of Arabidopsis. This enzyme specifically catalyzes the decomposition of Se-Cys into elemental Se and alanine. The resulting SL transgenics were shown to express the mouse enzyme in the expected intracellular location, and to have SL activities up to 2-fold (cytosolic lines) or 6-fold (chloroplastic lines) higher than wild-type plants. Se incorporation into proteins was reduced 2-fold in both types of SL transgenics, indicating that the approach successfully redirected Se flow in the plant. Both the cytosolic and chloroplastic SL plants showed enhanced shoot Se concentrations, up to 1.5-fold compared with wild type. The cytosolic SL plants showed enhanced tolerance to Se, presumably because of their reduced protein Se levels. Surprisingly, the chloroplastic SL transgenics were less tolerant to Se, indicating that (over) production of elemental Se in the chloroplast is toxic. Expression of SL in the cytosol may be a useful approach for the creation of plants with enhanced Se phytoremediation capacity.


1 This work was supported by the U.S. National Science Foundation (grant no. MCB-9982432 to E.A.H.P.-S. including a Research Experience for Undergraduates supplement to J.D.O., grant no. MCB-0091163 to M.P., and supplemental grant no. MCB-9982432 for international collaboration) and by a Grant-in-Aid for Joint Research Projects between Japan and the United States of America from the Japan Society for the Promotion of Science (to T.K.).

* Corresponding author; e-mail epsmits{at}lamar.colostate.edu; fax 970-491-0649.

© 2003 American Society of Plant Biologists



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