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Magnetic DNA affinity purification of yeast transcription factor tau--a new purification principle for the ultrarapid isolation of near homogeneous factor.

机译:酵母转录因子tau的磁性DNA亲和纯化-一种新的纯化原理用于近乎均质因子的超快速分离。

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摘要

We present a new method for rapid purification to near homogeneity of sequence specific DNA binding proteins based on magnetic separation. The method is described for the purification of the yeast transcription factor tau. DNA affinity Dynabeads (monodisperse superparamagnetic particles) specifically bind the protein in the presence of competitor DNA. By magnetic separation, wash and elution, highly enriched transcription factor preparations are obtained within minutes. In less than an hour with three cycles of adsorption, nearly homogeneous factor tau was obtained. The factor preparation contained mainly two polypeptides of 100 and 140 kDa and was fully active in transcription and DNA binding assays. This procedure should work for any high-affinity sequence-specific DNA binding protein with only minor modifications.
机译:我们提出了一种新方法,用于基于磁分离的序列特异性DNA结合蛋白的近乎同质的快速纯化。描述了用于纯化酵母转录因子tau的方法。 DNA亲和力Dynabeads(单分散超顺磁性颗粒)在竞争者DNA存在下特异性结合蛋白质。通过磁分离,洗涤和洗脱,可在数分钟内获得高度富集的转录因子制剂。在少于一个小时的三个吸附循环中,获得了几乎均一的因子tau。因子制剂主要包含两种100和140 kDa的多肽,并且在转录和DNA结合测定中具有完全活性。此过程仅需稍作修改即可适用于任何具有高亲和力的序列特异性DNA结合蛋白。

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