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Intein-mediated purification of cytotoxic endonuclease I-TevI by insertional inactivation and pH-controllable splicing

机译:通过插入失活和pH可控剪接,以内含肽介导的细胞毒性核酸内切酶I-TevI​​的纯化

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摘要

An intein-mediated approach was developed for expression and affinity purification of a protein that is lethal to Escherichia coli. The protein, I-TevI, is an intron-encoded endonuclease. The approach involved the insertional inactivation of I-TevI with a controllable mini-intein placed in front of a cysteine required for splicing (an I-TevI::intein fusion). The purification was facilitated by a chitin-binding domain inserted into the mini-intein. Affinity purification of the I-TevI::intein fusion precursor on a chitin column was followed by pH-controllable splicing to restore the structure and function of I-TevI. To study the impact of the insertion context on I-TevI inactivation, the chimeric intein was inserted independently in front of seven cysteines of I-TevI. One of the seven intein integrants yielded I-TevI of high activity. This technique is, in principle, generalizable to the expression and purification of other cytotoxic proteins and is amenable to scale-up.
机译:开发了一种内含肽介导的方法来表达和亲和纯化对大肠杆菌具有致死性的蛋白质。 I-TevI​​蛋白是内含子编码的核酸内切酶。该方法涉及将I-TevI​​插入插入失活,将可控制的微型内含肽置于剪接所需的半胱氨酸前面(I-TevI​​ :: intein融合蛋白)。插入迷你蛋白的几丁质结合结构域促进了纯化。亲和纯化甲壳质柱上的I-TevI​​ :: intein融合前体,然后进行pH可控的剪接,以恢复I-TevI​​的结构和功能。为了研究插入环境对I-TevI​​灭活的影响,将嵌合内含子独立插入I-TevI​​的七个半胱氨酸之前。七个内含肽整合剂之一产生了高活性的I-TevI​​。原则上,该技术可推广到其他细胞毒性蛋白的表达和纯化,并且可以扩大规模。

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