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A His-tag based immobilization method for the preparation and reconstitution of apoflavoproteins

机译:一种基于His标签的固定化方法,用于载脂蛋白的制备和重组

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摘要

The NifL PAS domain from Azotobacter vinelandii is a flavoprotein with FAD as the prosthetic group. Here we describe a novel immobilization procedure for the large-scale preparation of apo NifL PAS domain and its efficient reconstitution with either 2,4a-~(13)C)-FAD or 2,4a-~(13)C-FMN. In this procedure, the His-tagged holoprotein is bound to an immobilized metal affinity column and the flavin is released by washing the column with buffer containing 2 M KBr and 2 M urea. The apoprotein is reconstituted on-column with the (artificial) flavin cofactor, and then eluted with buffer containing 250 mM imidazole. Alternatively, the immobilized apoprotein can be released from the column matrix before reconstitution. The His-tag based immobilization method of preparing reconstituted (or apo) NifL PAS domain protein has the advantage that it combines a protein affinity chromatography technique with limited protein loss, resulting in a high protein yield with extremely efficient flavin reconstitution. This on-column reconstitution method can also be used in cases where the apoprotein is unstable. Therefore, it may develop as a universal method for replacement of flavin or other cofactors.
机译:来自葡萄固氮菌的NifL PAS结构域是一种以FAD为辅基的黄素蛋白。在这里,我们描述了用于大规模制备载脂蛋白NifL PAS结构域及其与2,4a-〜(13)C)-FAD或2,4a-〜(13)C-FMN的高效重组的新型固定程序。在此过程中,将带组氨酸标签的全蛋白结合到固定的金属亲和柱上,并用含有2 M KBr和2 M尿素的缓冲液洗涤该柱,从而释放出黄素。载脂蛋白与(人工)黄素辅因子在柱上重构,然后用含有250 mM咪唑的缓冲液洗脱。或者,固定的载脂蛋白可以在重构前从柱基质中释放出来。制备重组(或载脂蛋白)NafL PAS域蛋白的基于His-tag的固定化方法的优势在于,它结合了蛋白质亲和层析技术和有限的蛋白质损失,从而可实现高蛋白产量和极高效的黄素重构。在载脂蛋白不稳定的情况下,也可以使用这种柱上重建方法。因此,它可能会发展为取代黄素或其他辅因子的通用方法。

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