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Two mutations in the tetracycline repressor change the inducer anhydrotetracycline to a corepressor

机译:四环素阻遏物的两个突变将诱导剂脱水四环素转变为一个核心抑制剂

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摘要

We report for the first time the in vitro characterization of a reverse tetracycline repressor (revTetR). The dimeric wild-type repressor (TetR) binds to tet operator tetO in the absence of the inducer anhydrotetracycline (atc) to confer tight repression. We have isolated the revTetR G96E L205S mutant, which, contrary to TetR, binds tetO only in the presence of atc. This reverse acting mutant was overproduced and purified. Effector and DNA binding properties were analyzed by EMSA and quantified by fluorescence titration and surface plasmon resonance. The association constant KA of revTetR for binding of [atcMg]+ is ∼108 M–1, four orders of magnitude lower than that of TetR. The affinity of TetR for tetO is 5.6 ± 2 × 109 M–1 and that for revTetR in the presence of atc is 1 ± 0.2 × 108 M–1. Both induced forms, the atc-bound TetR and the free revTetR, have the same low affinity of 4 ± 1 × 105 M–1 for DNA. Therefore, atc does not act as a dimerization agent for revTetR. We discuss the structural differences between TetR and revTetR potentially underlying this reversal of activity.
机译:我们首次报告了反向四环素阻遏物(revTetR)的体外表征。在不存在诱导物脱水四环素(atc)的情况下,二聚体野生型阻遏物(TetR)与tet操纵子tetO结合,以提供严格的阻遏作用。我们已经分离出revTetR G96E L205S突变体,与TetR相反,该突变体仅在atc存在时才结合tetO。该反作用突变体被过量生产和纯化。通过EMSA分析效应子和DNA结合特性,并通过荧光滴定和表面等离振子共振进行定量。结合[atcMg] + 的revTetR的缔合常数KA为〜10 8 M -1 ,比其低4个数量级。 TetR。 TetR对tetO的亲和力为5.6±2×10 9 M –1 ,在atc存在下对revTetR的亲和力为1±0.2×10 8 < / sup> M –1 。两种诱导形式,即与atc结合的TetR和游离的revTetR,对DNA的亲和力均为4±1×10 5 M –1 。因此,atc不会充当revTetR的二聚剂。我们讨论了TetR和revTetR之间潜在的活动逆转的结构差异。

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