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A simple in vivo assay for increased protein solubility.

机译:一种简单的体内测定法用于增加蛋白质的溶解度。

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摘要

Low solubility is a major stumbling block in the detailed structural and functional characterization of many proteins and isolated protein domains. The production of some proteins in a soluble form may only be possible through alteration of their sequences by mutagenesis. The feasibility of this approach has been demonstrated in a number of cases where amino acid substitutions were shown to increase protein solubility without altering structure or function. However, identifying residues to mutagenize to increase solubility is difficult, especially in the absence of structural knowledge. For this reason, we have developed a method by which soluble mutants of an insoluble protein can be easily distinguished in vivo in Escherichia coli. This method is based on our observation that cells expressing fusions of an insoluble protein to chloramphenicol acetyltransferase (CAT) exhibit decreased resistance to chloramphenicol compared to fusions with soluble proteins. We found that a soluble mutant of an insoluble protein fused to CAT could be selected by plating on high levels of chloramphenicol.
机译:低溶解度是许多蛋白质和分离的蛋白质结构域的详细结构和功能表征中的主要绊脚石。只能通过诱变改变其序列来生产某些可溶形式的蛋白质。在许多情况下证明了这种方法的可行性,其中氨基酸取代已显示出增加蛋白质溶解度而不改变结构或功能的情况。但是,很难鉴定出要诱变以增加溶解度的残基,尤其是在缺乏结构知识的情况下。因此,我们已经开发出一种方法,通过该方法可以轻松地在大肠杆菌中在体内区分不溶蛋白的可溶性突变体。此方法基于我们的观察结果,即与可溶性蛋白融合蛋白相比,表达不溶蛋白与氯霉素乙酰转移酶(CAT)融合蛋白的细胞对氯霉素的抵抗力降低。我们发现可以通过在高水平的氯霉素上铺板来选择与CAT融合的不溶蛋白的可溶性突变体。

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