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Expression of the rDNA-encoded mitochondrial protein Tar1p is stringently controlled and responds differentially to mitochondrial respiratory demand and dysfunction

机译:严格控制rDNA编码的线粒体蛋白Tar1p的表达并对线粒体的呼吸需求和功能障碍做出不同的反应

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摘要

The novel yeast protein Tar1p is encoded on the anti-sense strand of the multi-copy nuclear 25S rRNA gene, localizes to mitochondria, and partially suppresses the mitochondrial RNA polymerase mutant, rpo41-R129D. However, the function of Tar1p in mitochondria and how its expression is regulated are currently unknown. Here we report that Tar1p is subject to glucose repression and is up-regulated during post-diauxic shift in glucose medium and in glycerol medium, conditions requiring elevated mitochondrial respiration. However, Tar1p expression is down-regulated in response to mitochondrial dysfunction caused by the rpo41-R129D mutation or in strains lacking respiration. Furthermore, in contrast to the previously reported beneficial effects of moderate over-expression of Tar1p in the rpo41-R129D strain, higher-level over-expression exacerbates the ROS-derived phenotypes of this mutant, including decreased respiration and life span. Finally, two-hybrid screening and in vitro-binding studies revealed a physical interaction between Tar1p and Coq5p, an enzyme involved in synthesizing the mitochondrial electron carrier and anti-oxidant, coenzyme Q. We propose that Tar1p expression is induced under respiratory conditions to maintain oxidative phosphorylation capacity, but that its levels in mitochondria are typically low and stringently controlled. Furthermore, we speculate that Tar1p is down-regulated when respiration is defective to prevent deleterious ROS-dependent consequences of mitochondrial dysfunction.
机译:新型酵母蛋白Tar1p在多拷贝核25S rRNA基因的反义链上编码,定位于线粒体,并部分抑制线粒体RNA聚合酶突变体rpo41-R129D。但是,目前尚不清楚Tar1p在线粒体中的功能及其表达调控方式。在这里,我们报告Tar1p受葡萄糖抑制,并且在葡萄糖介质和甘油介质中的diauxic转变过程中上调,条件是需要线粒体呼吸增加。但是,响应于由rpo41-R129D突变或缺乏呼吸的菌株引起的线粒体功能障碍,Tar1p表达下调。此外,与先前报道的rpo41-R129D菌株中Tar1p适度过表达的有益作用相反,更高水平的过表达加剧了该突变体的ROS衍生表型,包括呼吸和寿命降低。最后,通过两次杂交筛选和体外结合研究揭示了Tar1p和Coq5p之间的物理相互作用,该酶参与合成线粒体电子载体和抗氧化剂辅酶Q。我们建议在呼吸条件下诱导Tar1p表达,以维持氧化磷酸化能力,但其在线粒体中的水平通常较低且受到严格控制。此外,我们推测,当呼吸缺陷时,Tar1p会下调,以防止线粒体功能障碍的ROS依赖性有害后果。

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