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线粒体呼吸链复合物 I 的 NDUFB6 亚基是电子转移活性所必需的:在人细胞系中进行稳定和可控 RNA 干扰的原理验证研究。

The NDUFB6 subunit of the mitochondrial respiratory chain complex I is required for electron transfer activity: a proof of principle study on stable and controlled RNA interference in human cell lines.

机构信息

Inserm U676, Hôpital Robert Debré, F-75019 Paris, France.

出版信息

Biochem Biophys Res Commun. 2011 Oct 22;414(2):367-72. doi: 10.1016/j.bbrc.2011.09.078. Epub 2011 Sep 21.

DOI:10.1016/j.bbrc.2011.09.078
PMID:21964293
Abstract

Molecular bases of inherited deficiencies of mitochondrial respiratory chain complex I are still unknown in a high proportion of patients. Among 45 subunits making up this large complex, more than half has unknown function(s). Understanding the function of these subunits would contribute to our knowledge on mitochondrial physiology but might also reveal that some of these subunits are not required for the catalytic activity of the complex. A direct consequence of this finding would be the reduction of the number of candidate genes to be sequenced in patients with decreased complex I activity. In this study, we tested two different methods to stably extinct complex I subunits in cultured cells. We first found that lentivirus-mediated shRNA expression frequently resulted in the unpredicted extinction of additional gene(s) beside targeted ones. This can be ascribed to uncontrolled genetic material insertions in the genome of the host cell. This approach thus appeared inappropriate to study unknown functions of a gene. Next, we found it possible to specifically extinct a CI subunit gene by direct insertion of a miR targeting CI subunits in a Flp site (HEK293 Flp-In cells). By using this strategy we unambiguously demonstrated that the NDUFB6 subunit is required for complex I activity, and defined conditions suitable to undertake a systematic and stable extinction of the different supernumerary subunits in human cells.

摘要

遗传性线粒体呼吸链复合物 I 缺陷的分子基础在很大比例的患者中仍然未知。在构成这个大型复合物的 45 个亚基中,超过一半的亚基具有未知的功能。了解这些亚基的功能将有助于我们了解线粒体生理学,但也可能揭示出这些亚基中的一些对于复合物的催化活性不是必需的。这一发现的直接结果将是减少需要测序的候选基因数量在复合物 I 活性降低的患者中。在这项研究中,我们测试了两种稳定敲除培养细胞中复合物 I 亚基的不同方法。我们首先发现,慢病毒介导的 shRNA 表达经常导致除靶向外的其他基因的意外缺失。这可以归因于宿主细胞基因组中不受控制的遗传物质插入。因此,这种方法似乎不适合研究基因的未知功能。接下来,我们发现通过直接将靶向 CI 亚基的 miR 插入 Flp 位点(HEK293 Flp-In 细胞),可以特异性地敲除 CI 亚基基因。通过使用这种策略,我们明确证明了 NDUFB6 亚基对于复合物 I 活性是必需的,并确定了适合在人细胞中进行系统和稳定敲除不同多余亚基的条件。

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