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Mammalian metal response element-binding transcription factor-1 functions as a zinc sensor in yeast but not as a sensor of cadmium or oxidative stress

机译:哺乳动物金属反应元件结合转录因子-1充当酵母中的锌传感器但不充当镉或氧化应激的传感器

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摘要

The zinc finger protein, metal response element-binding transcription factor-1 (MTF-1) regulates the expression of genes in response to metal ions and oxidative stress. The precise mechanisms by which this occurs are not understood. To further examine this problem, mouse MTF-1 was expressed in Saccharomyces cerevisiae and tested for the ability to activate metal response element-driven reporter gene expression. Zinc was an effective inducer of reporter gene expression. In general, the magnitude of zinc induction was dependent on the concentration of zinc in the culture medium, but independent of the amount of MTF-1 expression. Zinc induction also occurred with either integrated or episomal reporter plasmids containing the native mouse metallothionein-I proximal promoter. Deletion of fingers 5 and 6 of MTF-1, which function in a zinc-dependent manner to stabilize the DNA-binding activity of the protein in vitro, did not diminish the zinc induction of either episomal or integrated promoters. However, a Gal4 DNA-binding domain– MTF-1 fusion protein, which binds constitutively to the Gal4-responsive promoter, was not zinc inducible but caused constitutive activation of reporter gene expression. This suggests that zinc activation of the DNA-binding activity of MTF-1 is the rate limiting step in its metalloregulatory function in yeast. In contrast, MTF-1 was not responsive to either cadmium or hydrogen peroxide, suggesting that distinct co-activators or signal transduction cascades not found in yeast are required to mediate MTF-1 activation of gene expression by this toxic metal and by oxidative stress.
机译:锌指蛋白,金属响应元件结合转录因子-1(MTF-1)调节基因的表达,以响应金属离子和氧化应激。发生这种情况的确切机制尚不清楚。为了进一步研究这个问题,在小鼠酿酒酵母中表达了小鼠MTF-1,并测试了其激活金属反应元件驱动的报道基因表达的能力。锌是报道基因表达的有效诱导物。通常,锌诱导的强度取决于培养基中锌的浓度,但与MTF-1表达量无关。含有天然小鼠金属硫蛋白-I近端启动子的整合型或游离型报道质粒也发生了锌诱导。 MTF-1的第5和第6指的删除以锌依赖性的方式起作用,以稳定蛋白质在体外的DNA结合活性,但并未减少游离型或整合型启动子对锌的诱导。但是,与Gal4反应性启动子组成性结合的Gal4 DNA结合域– MTF-1融合蛋白不是锌可诱导的,而是导致报告基因表达的组成性激活。这表明锌激活MTF-1的DNA结合活性是酵母中金属调控功能的限速步骤。相反,MTF-1对镉或过氧化氢均无反应,这表明需要通过酵母中未发现的独特的共激活因子或信号转导级联来介导这种有毒金属和氧化应激对基因表达的MTF-1激活。

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