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Myc Stimulates Nuclearly Encoded Mitochondrial Genes and Mitochondrial Biogenesis

机译:Myc刺激核编码的线粒体基因和线粒体的生物发生。

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Although several genes involved in mitochondrial function are direct Myc targets, the role of Myc in mitochondrial biogenesis has not been directly established. We determined the effects of ectopic Myc expression or the loss of Myc on mitochondrial biogenesis. Induction of Myc in P493-6 cells resulted in increased oxygen consumption and mitochondrial mass and function. Conversely, compared to wild-type Myc fibroblasts, Myc null rat fibroblasts have diminished mitochondrial mass and decreased number of normal mitochondria. Reconstitution of Myc expression in Myc null fibroblasts partially restored mitochondrial mass and function and normal-appearing mitochondria. Concordantly, we also observed in primary hepatocytes that acute deletion of floxed murine Myc by Cre recombinase resulted in diminished mitochondrial mass in primary hepatocytes. Our microarray analysis of genes responsive to Myc in human P493-6 B lymphocytes supports a role for Myc in mitochondrial biogenesis, since genes involved in mitochondrial structure and function are overrepresented among the Myc-induced genes. In addition to the known direct binding of Myc to many genes involved in mitochondrial structure and function, we found that Myc binds the TFAM gene, which encodes a key transcriptional regulator and mitochondrial DNA replication factor, both in P493-6 lymphocytes with high ectopic MYC expression and in serum-stimulated primary human 2091 fibroblasts with induced endogenous MYC. These observations support a pivotal role for Myc in regulating mitochondrial biogenesis.
机译:尽管参与线粒体功能的几个基因是Myc的直接靶标,但Myc在线粒体生物发生中的作用尚未直接建立。我们确定了异位Myc表达或 Myc 丢失对线粒体生物发生的影响。在P493-6细胞中诱导Myc导致耗氧量增加以及线粒体质量和功能的增加。相反,与野生型 Myc 成纤维细胞相比, Myc 无效大鼠成纤维细胞减少了线粒体质量,减少了正常线粒体的数量。在 Myc 空纤维母细胞中Myc表达的重建部分恢复了线粒体的质量和功能以及正常出现的线粒体。一致地,我们还观察到在原代肝细胞中,Cre重组酶对缺失的小鼠 Myc 的急性删除导致原代肝细胞线粒体质量的减少。我们对人类P493-6 B淋巴细胞中Myc响应的基因进行的微阵列分析支持Myc在线粒体生物发生中的作用,因为参与线粒体结构和功能的基因在Myc诱导的基因中过分代表。除了已知Myc与许多参与线粒体结构和功能的基因直接结合外,我们还发现Myc结合了 TFAM 基因,该基因编码P493中的关键转录调节因子和线粒体DNA复制因子。异位 MYC 表达高的-6淋巴细胞,以及内源性 MYC 诱导的血清刺激的原代人2091成纤维细胞。这些观察结果支持Myc在调节线粒体生物发生中的关键作用。

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