首页> 外文期刊>The Journal of biological chemistry >Selenocysteine Insertion at a Predefined UAG Codon in a Release Factor 1 (RF1)-depleted Escherichia coli Host Strain Bypasses Species Barriers in Recombinant Selenoprotein Translation
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Selenocysteine Insertion at a Predefined UAG Codon in a Release Factor 1 (RF1)-depleted Escherichia coli Host Strain Bypasses Species Barriers in Recombinant Selenoprotein Translation

机译:在释放因子1(RF1)耗尽的大肠杆菌宿主菌株中预先定义的UAG密码子的硒代半胱氨酸插入绕过重组硒蛋白翻译中的种类障碍。

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Selenoproteins contain the amino acid selenocysteine (Sec), co-translationally inserted at a predefined UGA opal codon by means of Sec-specific translation machineries. In Escherichia coli, this process is dependent upon binding of the Sec-dedicated elongation factor SelB to a Sec insertion sequence (SECIS) element in the selenoprotein-encoding mRNA and competes with UGA-directed translational termination. Here, we found that Sec can also be efficiently incorporated at a predefined UAG amber codon, thereby competing with RF1 rather than RF2. Subsequently, utilizing the RF1-depleted E. coli strain C321.ΔA, we could produce mammalian selenoprotein thioredoxin reductases with unsurpassed purity and yield. We also found that a SECIS element was no longer absolutely required in such a system. Human glutathione peroxidase 1 could thereby also be produced, and we could confirm a previously proposed catalytic tetrad in this selenoprotein. We believe that the versatility of this new UAG-directed production methodology should enable many further studies of diverse selenoproteins.
机译:硒蛋白包含氨基酸硒代半胱氨酸(Sec),通过Sec特异性翻译机制在预定的UGA蛋白石密码子上共翻译插入。在大肠杆菌中,此过程取决于Sec专用延伸因子SelB与编码硒蛋白的mRNA中Sec插入序列(SECIS)元件的结合,并与UGA定向的翻译终止竞争。在这里,我们发现Sec还可以有效地并入预定义的UAG琥珀色密码子,从而与RF1而非RF2竞争。随后,利用RF1耗尽的大肠杆菌C321.ΔA菌株,我们可以生产出纯度和产量均无与伦比的哺乳动物硒蛋白硫氧还蛋白还原酶。我们还发现,在这样的系统中,不再完全需要SECIS元素。人谷胱甘肽过氧化物酶1也可以由此产生,并且我们可以证实该硒蛋白中先前提出的催化四联体。我们认为,这种新的UAG指导的生产方法的多功能性应能使多种硒蛋白的进一步研究成为可能。

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