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Pptc7 is an essential phosphatase for promoting mammalian mitochondrial metabolism and biogenesis

机译:Pptc7是促进哺乳动物线粒体代谢和生物发生的必需磷酸酶。

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摘要

Mitochondrial proteins are replete with phosphorylation, yet its functional relevance remains largely unclear. The presence of multiple resident mitochondrial phosphatases, however, suggests that protein dephosphorylation may be broadly important for calibrating mitochondrial activities. To explore this, we deleted the poorly characterized matrix phosphatase Pptc7 from mice using CRISPR-Cas9 technology. Strikingly, Pptc7−/− mice exhibit hypoketotic hypoglycemia, elevated acylcarnitines and serum lactate, and die soon after birth. Pptc7−/− tissues have markedly diminished mitochondrial size and protein content despite normal transcript levels, and aberrantly elevated phosphorylation on select mitochondrial proteins. Among these, we identify the protein translocase complex subunit Timm50 as a putative Pptc7 substrate whose phosphorylation reduces import activity. We further find that phosphorylation within or near the mitochondrial targeting sequences of multiple proteins could disrupt their import rates and matrix processing. Overall, our data define Pptc7 as a protein phosphatase essential for proper mitochondrial function and biogenesis during the extrauterine transition.
机译:线粒体蛋白充满磷酸化,但其功能相关性仍不清楚。但是,存在多个驻留线粒体磷酸酶,这表明蛋白质去磷酸化对于校准线粒体活性可能具有广泛的重要性。为了探索这一点,我们使用CRISPR-Cas9技术从小鼠中删除了特征欠佳的基质磷酸酶Pptc7。引人注目的是,Pptc7 -/-小鼠表现出低酮症性低血糖,酰基肉碱和血清乳酸盐升高,并在出生后不久死亡。尽管转录本水平正常,但Pptc7 -/-组织的线粒体大小和蛋白质含量显着减少,并且某些线粒体蛋白质的磷酸化异常升高。在这些当中,我们确定了蛋白转运蛋白复合物亚基Timm50为推定的Pptc7底物,其磷酸化降低了进口活性。我们进一步发现,多种蛋白质的线粒体靶向序列内或附近的磷酸化可能破坏其导入率和基质加工。总的来说,我们的数据将Pptc7定义为在子宫外过渡过程中适当的线粒体功能和生物发生所必需的蛋白磷酸酶。

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