首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Synthesis of 5-methylaminomethyl-2-selenouridine in tRNAs: 31P NMR studies show the labile selenium donor synthesized by the selD gene product contains selenium bonded to phosphorus.
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Synthesis of 5-methylaminomethyl-2-selenouridine in tRNAs: 31P NMR studies show the labile selenium donor synthesized by the selD gene product contains selenium bonded to phosphorus.

机译:在tRNA中合成5-甲基氨基甲基-2-硒代尿苷:31P NMR研究表明由selD基因产物合成的不稳定的硒供体含有与磷结合的硒。

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摘要

An enzyme preparation from Salmonella typhimurium catalyzes the conversion of 5-methylaminomethyl-2-thiouridine in tRNAs to 5-methylaminomethyl-2-selenouridine when supplemented with selenide and ATP. Similar preparations from a Salmonella mutant strain carrying a defective selD gene fail to catalyze this selenium substitution reaction. However, supplementation of the deficient enzyme preparation with the purified selD gene product (SELD protein) restored synthesis of seleno-tRNAs. In the absence of the complementary enzyme(s), the SELD protein catalyzes the synthesis of a labile selenium donor compound from selenide and ATP. 31P NMR studies show that among the products of this reaction are AMP and a compound containing selenium bonded to phosphorus. The reaction is completely dependent on the addition of both selenide and magnesium. The dependence of reaction velocity on ATP concentration shows sigmoidal kinetics, whereas dependence on selenide concentration obeys Michaelis-Menten kinetics indicating a Km value of 46 microM for selenide.
机译:当补充硒化物和ATP时,鼠伤寒沙门氏菌的酶制剂可催化tRNA中的5-甲基氨基甲基-2-硫尿苷转化为5-甲基氨基甲基-2-硒代尿苷。携带有缺陷的selD基因的沙门氏菌突变株的类似制剂无法催化这种硒取代反应。但是,用纯化的selD基因产物(SELD蛋白)补充有缺陷的酶制剂可恢复硒代tRNA的合成。在不存在互补酶的情况下,SELD蛋白催化由硒化物和ATP合成不稳定的硒供体化合物。 31 P NMR研究表明,该反应的产物中有AMP和一种与磷结合的含硒化合物。该反应完全取决于硒化物和镁的添加。反应速度对ATP浓度的依赖性呈S形动力学,而对硒化物浓度的依赖性符合Michaelis-Menten动力学,表明硒化物的Km值为46 microM。

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