首页> 美国卫生研究院文献>Protein Science : A Publication of the Protein Society >Expression of a soluble form of iodotyrosine deiodinase for active site characterization by engineering the native membrane protein from Mus musculus
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Expression of a soluble form of iodotyrosine deiodinase for active site characterization by engineering the native membrane protein from Mus musculus

机译:通过改造小家鼠的天然膜蛋白表达可溶形式的碘酪氨酸脱碘酶以进行活性位点鉴定

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摘要

Reductive deiodination is critical for thyroid function and represents an unusual exception to the more common oxidative and hydrolytic mechanisms of dehalogenation in mammals. Studies on the reductive processes have been limited by a lack of convenient methods for heterologous expression of the appropriate proteins in large scale. The enzyme responsible for iodide salvage in the thyroid, iodotyrosine deodinase, is now readily generated after engineering its gene from Mus musculus. High expression of a truncated derivative lacking the membrane domain at its N-terminal was observed in Sf9 cells, whereas expression in Pichia pastoris remained low despite codon optimization. Ultimately, the desired expression in Escherichia coli was achieved after replacing the two conserved Cys residues of the deiodinase with Ala and fusing the resulting protein to thioredoxin. This final construct provided abundant enzyme for crystallography and mutagenesis. Utility of the E. coli system was demonstrated by examining a set of active site residues critical for binding to the zwitterionic portion of substrate.
机译:还原性脱碘对于甲状腺功能至关重要,它代表了哺乳动物脱卤中较常见的氧化和水解机制的一个异常例外。由于缺乏合适的大规模异源表达蛋白的简便方法,还原过程的研究受到了限制。在从小家鼠中改造其基因后,现在很容易生成负责甲状腺中碘化物挽救的酶碘酪氨酸脱碘酶。在Sf9细胞中观察到了在N末端缺少膜结构域的截短的衍生物的高表达,尽管有密码子优化,但在毕赤酵母中的表达仍然很低。最终,在将脱碘酶的两个保守的Cys残基替换为Ala并将所得蛋白质融合到硫氧还蛋白上后,在大肠杆菌中获得了所需的表达。这种最终的构建体为结晶学和诱变提供了丰富的酶。通过检查一组对结合底物的两性离子部分至关重要的活性位点残基证明了大肠杆菌系统的实用性。

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