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Miro1-mediated mitochondrial positioning shapes intracellular energy gradients required for cell migration

机译:miro1介导的线粒体定位形状细胞迁移所需的细胞内能量梯度

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It has long been postulated, although never directly demonstrated, that mitochondria are strategically positioned in the cytoplasm to meet local requirements for energy production. Here we show that positioning of mitochondria in mouse embryonic fibroblasts (MEFs) determines the shape of intracellular energy gradients in living cells. Specifically, the ratio of ATP to ADP was highest at perinuclear areas of dense mitochondria and gradually decreased as more-peripheral sites were approached. Furthermore, the majority of mitochondria were positioned at the ventral surface of the cell, correlating with high ATP: ADP ratios close to the ventral membrane, which rapidly decreased toward the dorsal surface. We used cells deficient for the mitochondrial Rho-GTPase 1 (Miro1), an essential mediator of microtubule-based mitochondrial motility, to study how changes in mitochondrial positioning affect cytoplasmic energy distribution and cell migration, an energy-expensive process. The mitochondrial network in Miro1(-/-) MEFs was restricted to the perinuclear area, with few mitochondria present at the cell periphery. This change in mitochondrial distribution dramatically reduced the ratio of ATP to ADP at the cell cortex and disrupted events essential for cell movement, including actin dynamics, lamellipodia protrusion, and membrane ruffling. Cell adhesion status was also affected by changes in mitochondrial positioning; focal adhesion assembly and stability was decreased in Miro1(-/-) MEFs compared with Miro1(+/+) MEFs. Consequently Miro1(-/-) MEFs migrated slower than control cells during both collective and single-cell migration. These data establish that Miro1-mediated mitochondrial positioning at the leading edge provides localized energy production that promotes cell migration by supporting membrane protrusion and focal adhesion stability.
机译:它已经长期假设,虽然从未直接证明过,线粒体在细胞质中策略性地定位,以满足能源生产的当地要求。在这里,我们表明线粒体在小鼠胚胎成纤维细胞(MEFS)中的定位决定了活细胞中细胞内能量梯度的形状。具体地,在致密线粒体的PerinuclecleclecthondRia的Perinuclecleclecar核区域中,ATP与ADP的比率最高,并且随着更多外周位点逐渐降低。此外,大多数线粒体定位在细胞的腹表面,与高ATP的相关性:靠近腹膜的ADP比,这朝向背面迅速降低。我们使用缺乏线粒体Rho-GTPAse1(Miro1)的细胞,基于微管的线粒体运动的基本介体,研究线粒体定位的变化如何影响细胞质能量分布和细胞迁移,是一种能量昂贵的方法。 Miro1( - / - )MEF中的线粒体网络仅限于细胞周边存在少量线粒体。线粒体分布的这种变化显着降低了在细胞皮层的ATP与ADP的比例,并破坏了对细胞运动,包括肌动蛋白动力学,层状动力学和膜荷丝卷曲。细胞粘附状态也受线粒体定位变化的影响;与Miro1(+ / +)MEF相比,Miro1( - / - )MEF中的焦粘性组件和稳定性降低。因此,Miro1( - / - )MEF在集体和单细胞迁移过程中迁移比控制单元慢。这些数据在前缘确定Miro1介导的线粒体定位提供通过支撑膜突起和局灶性粘附稳定性来促进细胞迁移的局部能量产生。

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