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Methylthioadenosine and polyamine biosynthesis in a Saccharomyces cerevisiae meu1delta mutant.

机译:酿酒酵母meu1delta突变体中的甲硫基腺苷和多胺的生物合成。

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摘要

As part of our studies on polyamine biosynthesis in yeast, the metabolism of methylthioadenosine was studied in a mutant that lacks methylthioadenosine phosphorylase (meu1delta). The nucleoside accumulates in this mutant and is mainly excreted into the culture medium. Intracellular accumulation of the nucleoside is enough to account for the inhibition of spermidine synthase and thus to indirectly regulate the polyamine content of the meu1delta cells. By comparing the results with this mutant with a meu1delta spe2delta mutant that cannot synthesize spermidine or spermine, we showed that >98% of methylthioadenosine is produced as a byproduct of polyamine synthesis (i.e., from decarboxylated S-adenosylmethionine). In contrast, in MEU1+ SPE2+ cells methylthioadenosine does not accumulate and is metabolized through the methionine salvage pathway. Using a met15delta mutant we show that this pathway (i.e., involving polyamine biosynthesis and methylthioadenosine metabolism) is a significant factor in the metabolism of methionine, accounting for 15% of the added methionine.
机译:作为我们关于酵母中多胺生物合成的研究的一部分,在缺少甲基硫代腺苷磷酸化酶(meu1delta)的突变体中研究了甲基硫代腺苷的代谢。核苷在该突变体中积累,并且主要排泄到培养基中。核苷的细胞内积累足以说明对亚精胺合酶的抑制作用,因此间接调节了meu1delta细胞的多胺含量。通过将该结果与无法合成亚精胺或亚精胺的meu1delta spe2delta突变体进行比较,我们表明多聚体合成的副产物(即由脱羧化S-腺苷甲硫氨酸)产生了98%以上的甲硫基腺苷。相反,在MEU1 + SPE2 +细胞中,甲硫基腺苷不会积聚,而是通过蛋氨酸抢救途径代谢。使用met15delta突变体,我们表明该途径(即涉及多胺生物合成和甲硫基腺苷代谢)是蛋氨酸代谢的重要因素,占蛋氨酸添加量的15%。

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