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Purification of DNA-binding transcription factors by their selective adsorption on the affinity latex particles.

机译:通过将DNA结合转录因子选择性吸附在亲和性乳胶颗粒上来进行纯化。

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摘要

A simple method with the use of affinity latex particles has been developed for the fast and efficient purification of sequence-specific DNA-binding proteins on the basis of their ability to selectively bind to their target sequences. Complementary oligodeoxynucleotides that contained a recognition site for a sequence-specific DNA-binding protein were chemically synthesized, annealed and ligated to give oligomers. The oligomers were coupled to latex particles, composed of polyglycidyl methacrylate, using cyanogen bromide to yield affinity latex particles. The concentration of covalently bound DNA on the affinity latex particles was 6 times as much DNA per ml as that in the Sepharose resin conventionally used. By sequential batch-wise procedures with the affinity particles, one of the sequence-specific DNA binding transcription factors, ATF or E4TF3, was quickly and efficiently purified to homogeneity from either a protein fraction in which the factor was enriched or a crude cell extract.
机译:已经开发出一种使用亲和乳胶颗粒的简单方法,用于根据其选择性结合其靶序列的能力快速有效地纯化序列特异性DNA结合蛋白。化学合成,退火并连接包含序列特异性DNA结合蛋白识别位点的互补寡聚脱氧核苷酸,得到寡聚体。使用溴化氰将低聚物偶联至由聚甲基丙烯酸缩水甘油酯组成的胶乳颗粒,以产生亲和力的胶乳颗粒。亲和力胶乳颗粒上共价结合的DNA的浓度是每毫升DNA的6倍,是常规使用的Sepharose树脂中DNA的浓度的6倍。通过使用亲和颗粒的连续分批程序,可以从其中富集因子的蛋白质馏分或粗制细胞提取物中快速,有效地纯化序列特异性DNA结合转录因子之一ATF或E4TF3,使其达到均质。

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