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Nucleolin binds to a subset of selenoprotein mRNAs and regulates their expression.

机译:核仁蛋白与硒蛋白mRNA的一个子集结合并调节其表达。

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摘要

Selenium, an essential trace element, is incorporated into selenoproteins as selenocysteine (Sec), the 21st amino acid. In order to synthesize selenoproteins, a translational reprogramming event must occur since Sec is encoded by the UGA stop codon. In mammals, the recoding of UGA as Sec depends on the selenocysteine insertion sequence (SECIS) element, a stem-loop structure in the 3' untranslated region of the transcript. The SECIS acts as a platform for RNA-binding proteins, which mediate or regulate the recoding mechanism. Using UV crosslinking, we identified a 110 kDa protein, which binds with high affinity to SECIS elements from a subset of selenoprotein mRNAs. The crosslinking activity was purified by RNA affinity chromatography and identified as nucleolin by mass spectrometry analysis. In vitro binding assays showed that purified nucleolin discriminates among SECIS elements in the absence of other factors. Based on siRNA experiments, nucleolin is required for the optimal expression of certain selenoproteins. There was a good correlation between the affinity of nucleolin for a SECIS and its effect on selenoprotein expression. As selenoprotein transcript levels and localization did not change in siRNA-treated cells, our results suggest that nucleolin selectively enhances the expression of a subset of selenoproteins at the translational level.
机译:硒是必需的微量元素,被作为硒代半胱氨酸(Sec)(第21个氨基酸)掺入硒蛋白中。为了合成硒蛋白,由于Sec由UGA终止密码子编码,因此必须发生翻译重编程事件。在哺乳动物中,UGA的Sec编码取决于硒代半胱氨酸插入序列(SECIS)元件,即转录物3'非翻译区的茎环结构。 SECIS作为RNA结合蛋白的平台,介导或调节编码机制。使用紫外线交联,我们确定了一个110 kDa的蛋白,该蛋白与硒蛋白mRNA子集中的SECIS元素具有高亲和力。通过RNA亲和层析纯化交联活性,并通过质谱分析鉴定为核仁素。体外结合试验表明,在没有其他因素的情况下,纯化的核仁素可在SECIS元素之间进行区分。根据siRNA实验,需要核仁素才能最佳表达某些硒蛋白。核仁素对SECIS的亲和力及其对硒蛋白表达的影响之间具有良好的相关性。由于在siRNA处理的细胞中硒蛋白的转录水平和定位没有变化,因此我们的结果表明,核仁蛋白在翻译水平上选择性地增强了硒蛋白亚型的表达。

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