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ATP 合酶亚基 9 mRNA 的局部翻译改变了轴突中的 ATP 水平和 ROS 的产生。

Local translation of ATP synthase subunit 9 mRNA alters ATP levels and the production of ROS in the axon.

机构信息

Laboratory of Molecular Biology, National Institute of Mental Health, National Institutes of Health, Bethesda, MD 20892-1381, USA.

出版信息

Mol Cell Neurosci. 2012 Mar;49(3):263-70. doi: 10.1016/j.mcn.2011.12.006. Epub 2011 Dec 21.

Abstract

To date, it has been demonstrated that axonal mRNA populations contain a large number of nuclear-encoded mRNAs for mitochondrial proteins. Here, we report that the mRNA encoding ATP synthase subunit 9 (ATP5G1), a key component of Complex V of the oxidative phosphorylation chain, is present in the axons of rat primary sympathetic neurons, as judged by in situ hybridization and qRT-PCR methodology. Results of metabolic labeling studies establish that this nuclear-encoded mRNA is translated in the axon. The siRNA-mediated knock-down of axonal ATP5G1 mRNA resulted in a significant reduction of axonal ATP5G1 protein and ATP levels. Silencing of local ATP5G1 expression enhanced the production of local reactive oxygen species (ROS). Importantly, reduction in the levels of ATP5G1 expression resulted in a marked attenuation in the rate of elongation of the axon. Exposure of the distal axons to nordihydroguaiaretic acid (NDGA), a ROS scavenger, mitigated the reduction in the rate of axon elongation observed after knock-down of ATP5G1. Taken together, these data call attention to the key regulatory role that local translation of nuclear-encoded mitochondrial mRNAs plays in energy metabolism and growth of the axon.

摘要

迄今为止,已经证明轴突 mRNA 群体包含大量核编码的线粒体蛋白的 mRNA。在这里,我们报告说,编码 ATP 合酶亚基 9(ATP5G1)的 mRNA,氧化磷酸化链复合物 V 的关键组成部分,存在于大鼠原代交感神经元的轴突中,这可以通过原位杂交和 qRT-PCR 方法来判断。代谢标记研究的结果确定,这种核编码的 mRNA 在轴突中被翻译。通过 siRNA 介导的敲低轴突 ATP5G1 mRNA,导致轴突 ATP5G1 蛋白和 ATP 水平显著降低。轴突局部 ATP5G1 表达的沉默增强了局部活性氧物质 (ROS) 的产生。重要的是,降低 ATP5G1 表达水平导致轴突伸长率明显降低。将远端轴突暴露于 Nordihydroguaiaretic acid(NDGA),一种 ROS 清除剂,减轻了敲低 ATP5G1 后观察到的轴突伸长率降低。总之,这些数据引起了人们对核编码线粒体 mRNA 的局部翻译在轴突能量代谢和生长中所起的关键调节作用的关注。

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