Ogasawara Yuki, Lacourciere Gerard M, Ishii Kazuyuki, Stadtman Thressa C
Department of Environmental Biology, Meiji Pharmaceutical University, 2-522-1 Noshio, Kiyose, Nishitokyo, Tokyo 204-8588, Japan.
Proc Natl Acad Sci U S A. 2005 Jan 25;102(4):1012-6. doi: 10.1073/pnas.0409042102. Epub 2005 Jan 14.
Selenophosphate, an activated form of selenium that can serve as a selenium donor, is generated by the selD gene product, selenophosphate synthetase (SPS). Selenophosphate is required by several bacteria and by mammals for the specific synthesis of Secys-tRNA, the precursor of selenocysteine in selenoenzymes. Although free selenide can be used in vitro for synthesis of selenophosphate, the physiological system that donates selenium to SPS is incompletely characterized. To detect potential selenium-delivery proteins, two known sulfurtransferases and glyceraldehyde-3-phosphate dehydrogenase (GAPDH; EC 1.2.1.12) were analyzed for ability to bind and transfer selenium. Rhodanese (EC 2.8.1.1) was shown to bind selenium tightly, with only part of the selenium being available as substrate for SPS in the presence of added reductant. 3-Mercaptopyruvate sulfurtransferase (3-MST; EC 2.8.1.2) and GAPDH also bound selenium supplied as selenodiglutathione formed from SeO3(2-) and glutathione. Selenium bound to 3-MST and GAPDH was released more readily than that from rhodanese and also was more available as a substrate for SPS. Although rhodanese retained tightly bound selenium under aerobic conditions, the protein gradually became insoluble, whereas GAPDH containing bound selenium was stable at neutral pH for a long period. These results indicate that 3-MST and GAPDH have more suitable potentials as a physiological selenium-delivery protein than rhodanese. In the presence of a selenium-binding protein, a low level of selenodiglutathione formed from SeO3(2-) and glutathione could effectively replace the high concentrations of selenide routinely used as substrate in the SPS in vitro assays.
硒代磷酸酯是硒的一种活化形式,可作为硒供体,由selD基因产物硒代磷酸酯合成酶(SPS)产生。几种细菌和哺乳动物在特异性合成硒代半胱氨酸-tRNA(硒酶中硒代半胱氨酸的前体)时需要硒代磷酸酯。尽管游离硒化物可在体外用于合成硒代磷酸酯,但向SPS提供硒的生理系统尚未完全明确。为了检测潜在的硒传递蛋白,分析了两种已知的硫转移酶和甘油醛-3-磷酸脱氢酶(GAPDH;EC 1.2.1.12)结合和转移硒的能力。硫氰酸酶(EC 2.8.1.1)被证明能紧密结合硒,在添加还原剂的情况下,只有部分硒可作为SPS的底物。3-巯基丙酮酸硫转移酶(3-MST;EC 2.8.1.2)和GAPDH也能结合由SeO3(2-)和谷胱甘肽形成的硒代二谷胱甘肽提供的硒。与硫氰酸酶相比,结合在3-MST和GAPDH上的硒释放得更容易,也更易作为SPS的底物。尽管硫氰酸酶在有氧条件下能保留紧密结合的硒,但该蛋白会逐渐变得不溶,而含有结合硒的GAPDH在中性pH下能长期保持稳定。这些结果表明,与硫氰酸酶相比,3-MST和GAPDH作为生理硒传递蛋白具有更合适的潜力。在存在硒结合蛋白的情况下,由SeO3(2-)和谷胱甘肽形成的低水平硒代二谷胱甘肽可有效替代体外SPS测定中常规用作底物的高浓度硒化物。