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链霉亲和素标签II亲和纯化:一种研究金属酶生物合成中间体的方法。

Strep-tag II affinity purification: an approach to study intermediates of metalloenzyme biosynthesis.

作者信息

Maier T, Drapal N, Thanbichler M, Böck A

机构信息

Lehrstuhl für Mikrobiologie, Universität München, Munich, Germany.

出版信息

Anal Biochem. 1998 May 15;259(1):68-73. doi: 10.1006/abio.1998.2649.

Abstract

Complex metalloenzymes (e.g., nitrogenase, hydrogenase, urease) are synthesized starting from the apoprotein via several intermediates by the action of accessory proteins. The isolation and biochemical characterization of such intermediates is hampered by their low abundance and their lability. Here we describe a technique for efficient single-step purification of a hydrogenase precursor under mild conditions using a N-terminal Strep-tag II affinity peptide and a novel StrepTactin Sepharose matrix. The tag was fused to the large subunit of [NiFe] hydrogenase 3 (HycE) of Escherichia coli. No significant influence of the affinity peptide on maturation or activity of the protein was observed when the modified gene was integrated into the chromosome by homologous recombination. A tagged nickel-free precursor form of HycE bound quantitatively to a recombinant StrepTactin Sepharose column. More than 90% pure subunit could be obtained after elution with desthiobiotin. The procedure was shown to be more efficient than purification by immobilized metal affinity chromatography using a N-terminal His-tag. General advantages of the novel Strep-tag II affinity purification especially for applications with metalloenzymes are discussed.

摘要

复杂金属酶(如固氮酶、氢化酶、脲酶)是通过辅助蛋白的作用,从脱辅基蛋白开始,经过几种中间体合成的。这些中间体的低丰度和不稳定性阻碍了它们的分离和生化特性研究。在此,我们描述了一种在温和条件下,使用N端链霉亲和标签II亲和肽和新型链霉抗生物素蛋白琼脂糖基质,对氢化酶前体进行高效单步纯化的技术。该标签与大肠杆菌[NiFe]氢化酶3(HycE)的大亚基融合。当通过同源重组将修饰基因整合到染色体中时,未观察到亲和肽对蛋白质成熟或活性有显著影响。带有标签的无镍HycE前体形式定量结合到重组链霉抗生物素蛋白琼脂糖柱上。用脱硫生物素洗脱后可获得纯度超过90%的亚基。结果表明,该方法比使用N端组氨酸标签的固定化金属亲和色谱纯化更有效。讨论了新型链霉亲和标签II亲和纯化的一般优势,特别是在金属酶应用方面。

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