Joseph Anna-Maria, Rungi Arne A, Robinson Brian H, Hood David A
Department of Biology, York University, Toronto, Canada M3J IP3.
Am J Physiol Cell Physiol. 2004 Apr;286(4):C867-75. doi: 10.1152/ajpcell.00191.2003. Epub 2003 Dec 3.
Defects in mitochondrial DNA (mtDNA) evoke distinctive responses in the nuclear genome, leading to altered mitochondrial biogenesis. We used C(2)C(12) cells depleted of mtDNA (rho(-) cells) and fibroblasts from a mitochondrial encephalopathy, lactic acidosis, and strokelike episodes (MELAS) patient to examine adaptations of the protein import machinery and transcription factors involved in mitochondrial biogenesis. In rho(-) cells, Tom20 and Tim23 protein levels were reduced by 25% and 59%, whereas mtHSP70 was induced by twofold relative to control cells. These changes were accompanied by a 21% increase in enhanced yellow fluorescent protein (EYFP) import into mitochondria in rho(-) cells (P < 0.05). In contrast, in MELAS cells mtHSP70 was elevated by 70%, whereas Tom20 and Tom34 protein levels were increased by 45% and 112% relative to control values. EYFP import was not altered in MELAS cells. In rho(-) cells, protein levels of the transcription factors nuclear respiratory factor-1 (NRF-1) and transcription factor A (Tfam) declined by 33% and 54%, whereas no change was observed for the coactivator peroxisome proliferator receptor-gamma coactivator-1alpha (PGC-1alpha). In contrast, Tfam was increased by 40% in MELAS cells. Rho(-) cells displayed reduced oxygen consumption (Vo(2)) and ATP levels, along with a twofold increase in lactate levels (P < 0.05). In electrically stimulated C(2)C(12) cells, 109%, 78%, 60%, and 67% increases were observed in mtDNA, Vo(2), cytochrome-c oxidase (COX) activity, and Tom34 levels, respectively (P < 0.05). Our findings suggest that compensatory adaptations occurred to maintain normal rates of protein import in response to mtDNA defects and support a role for contractile activity in reducing pathophysiology associated with mtDNA depletion. Because the expression of nuclear-encoded transcription factors and protein import machinery components was dependent on the type of mtDNA defect, these findings suggest involvement of distinct signaling cascades, each dependent on the type of mitochondrial defect, resulting in divergent changes in nuclear gene expression patterns.
线粒体DNA(mtDNA)缺陷会在核基因组中引发独特的反应,导致线粒体生物合成发生改变。我们使用缺乏mtDNA的C(2)C(12)细胞(ρ⁻细胞)以及一名患有线粒体脑肌病、乳酸酸中毒和卒中样发作(MELAS)患者的成纤维细胞,来研究参与线粒体生物合成的蛋白质导入机制和转录因子的适应性变化。在ρ⁻细胞中,Tom20和Tim23的蛋白质水平分别降低了25%和59%,而mtHSP70相对于对照细胞被诱导增加了两倍。这些变化伴随着增强型黄色荧光蛋白(EYFP)导入ρ⁻细胞线粒体的量增加了21%(P < 0.05)。相比之下,在MELAS细胞中,mtHSP70升高了70%,而Tom20和Tom34的蛋白质水平相对于对照值分别增加了45%和112%。MELAS细胞中EYFP的导入没有改变。在ρ⁻细胞中,转录因子核呼吸因子-1(NRF-1)和转录因子A(Tfam)的蛋白质水平分别下降了33%和54%,而共激活因子过氧化物酶体增殖物激活受体γ共激活因子-1α(PGC-1α)没有变化。相比之下,MELAS细胞中Tfam增加了40%。ρ⁻细胞的氧消耗(Vo₂)和ATP水平降低,乳酸水平增加了两倍(P < 0.05)。在电刺激的C(2)C(12)细胞中,mtDNA、Vo₂、细胞色素c氧化酶(COX)活性和Tom34水平分别增加了109%、78%、60%和67%(P < 0.05)。我们的研究结果表明,为应对mtDNA缺陷,发生了代偿性适应以维持正常的蛋白质导入速率,并支持收缩活动在减轻与mtDNA耗竭相关的病理生理过程中的作用。由于核编码转录因子和蛋白质导入机制成分的表达取决于mtDNA缺陷的类型,这些发现表明存在不同的信号级联反应,每个反应都取决于线粒体缺陷的类型,导致核基因表达模式发生不同的变化。
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