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Regulation of Selenocysteine Incorporation into the Selenium Transport Protein Selenoprotein P

机译:硒代半胱氨酸掺入硒转运蛋白硒蛋白P的调控

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摘要

Selenoproteins are unique as they contain selenium in their active site in the form of the 21st amino acid selenocysteine (Sec), which is encoded by an in-frame UGA stop codon. Sec incorporation requires both cis- and trans-acting factors, which are known to be sufficient for Sec incorporation in vitro, albeit with low efficiency. However, the abundance of the naturally occurring selenoprotein that contains 10 Sec residues (SEPP1) suggests that processive and efficient Sec incorporation occurs in vivo. Here, we set out to study native SEPP1 synthesis in vitro to identify factors that regulate processivity and efficiency. Deletion analysis of the long and conserved 3′-UTR has revealed that the incorporation of multiple Sec residues is inherently processive requiring only the SECIS elements but surprisingly responsive to the selenium concentration. We provide evidence that processive Sec incorporation is linked to selenium utilization and that reconstitution of known Sec incorporation factors in a wheat germ lysate does not permit multiple Sec incorporation events, thus suggesting a role for yet unidentified mammalian-specific processes or factors. The relationship between our findings and the channeling theory of translational efficiency is discussed.
机译:硒蛋白是独特的,因为它们在活性位点以第21个氨基酸硒代半胱氨酸(Sec)的形式包含硒,该硒由一个读码框内的UGA终止密码子编码。 Sec掺入需要顺式和反式作用因子,尽管效率低,但已知这足以在体外进行Sec掺入。但是,包含10个Sec残基(SEPP1)的天然存在的硒蛋白丰富表明体内进行了有效的Sec掺入。在这里,我们着手研究天然SEPP1的体外合成,以识别调节生产力和效率的因素。对长且保守的3'-UTR的缺失分析表明,多个Sec残基的掺入本质上是过程性的,仅需要SECIS元素,但是出人意料地对硒浓度作出响应。我们提供的证据表明,过程性Sec掺入与硒利用有关,并且已知的Sec掺入因子在小麦胚芽裂解物中的重构不允许发生多个Sec掺入事件,因此暗示了尚未确定的哺乳动物特异性过程或因素的作用。讨论了我们的发现与翻译效率的引导理论之间的关系。

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