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Modulation of myosin A expression by a newly established tetracycline repressor-based inducible system in Toxoplasma gondii

机译:刚建立的基于弓形体的基于四环素阻遏物的诱导系统对肌球蛋白A表达的调节

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摘要

We have developed a control system for regulating gene activation in Toxoplasma gondii. The elements of this system are derived from the Escherichia coli tetracycline resistance operon, which has been widely used to tightly control gene expression in eukaryotes. The tetracycline repressor (tetR) interferes with transcription initiation while the chimeric transactivator, composed of the tetR fused to the activating domain of VP16 transcriptional factor, allows tet-dependent transcription. Accordingly, tetracycline derivatives such as anhydrotetracycline, which we found to be well tolerated by T.gondii, can serve as effector molecules, allowing control of gene expression in a reversible manner. As a prerequisite to functionally express the tetR in T.gondii, we used a synthetic gene with change of codon frequency. Whereas no activation of transcription was achieved using the synthetic tetracycline-controlled transactivator, tTA2s, the TetRs modulates parasite transcription over a range of ~15-fold as measured for several reporter genes. We show here that the tetR-dependent induction of the T.gondii myosin A transgene expression drastically down-regulates the level of endogenous MyoA. This myosin is under the control of a tight feedback mechanism, which occurs at the protein level.
机译:我们已经开发了一个控制系统,用于调节弓形虫中的基因激活。该系统的元素源自大肠杆菌四环素抗性操纵子,该操纵子已被广泛用于严格控制真核生物中的基因表达。四环素阻遏物(tetR)干扰转录启动,而由与VP16转录因子激活域融合的tetR组成的嵌合反式激活子允许tet依赖性转录。相应地,我们发现T.gondii对四环素衍生物如脱水四环素具有很好的耐受性,它可以作为效应分子,以可逆方式控制基因表达。作为在T.gondii中功能表达tetR的先决条件,我们使用了具有密码子频率变化的合成基因。使用合成的四环素控制的反式激活剂tTA2 s 不能实现转录激活,而TetR s 可以在约15倍的范围内调节寄生虫的转录,这是对几种方法的测量报告基因。我们在这里显示T.gondii肌球蛋白A转基因表达的tetR依赖性诱导显着下调内源性MyoA的水平。该肌球蛋白在紧密的反馈机制的控制下,该机制发生在蛋白质水平。

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