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MGME1 processes flaps into ligatable nicks in concert with DNA polymerase γ during mtDNA replication

机译:MGME1在mtDNA复制过程中与DNA聚合酶γ协同作用将襟翼加工成可韧带的切口

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摘要

Recently, MGME1 was identified as a mitochondrial DNA nuclease with preference for single-stranded DNA (ssDNA) substrates. Loss-of-function mutations in patients lead to mitochondrial disease with DNA depletion, deletions, duplications and rearrangements. Here, we assess the biochemical role of MGME1 in the processing of flap intermediates during mitochondrial DNA replication using reconstituted systems. We show that MGME1 can cleave flaps to enable efficient ligation of newly replicated DNA strands in combination with POLγ. MGME1 generates a pool of imprecisely cut products (short flaps, nicks and gaps) that are converted to ligatable nicks by POLγ through extension or excision of the 3′-end strand. This is dependent on the 3′-5′ exonuclease activity of POLγ which limits strand displacement activity and enables POLγ to back up to the nick by 3′-5′ degradation. We also demonstrate that POLγ-driven strand displacement is sufficient to generate DNA- but not RNA-flap substrates suitable for MGME1 cleavage and ligation during replication. Our findings have implications for RNA primer removal models, the 5′-end processing of nascent DNA at OriH, and DNA repair.
机译:最近,MGME1被鉴定为线粒体DNA核酸酶,偏向于单链DNA(ssDNA)底物。患者的功能丧失突变会导致线粒体疾病,并伴有DNA耗尽,缺失,重复和重排。在这里,我们评估MGME1在使用重组系统的线粒体DNA复制过程中皮瓣中间体的加工中的生化作用。我们表明,MGME1可以裂解皮瓣,使有效复制的新复制的DNA链与POLγ结合。 MGME1生成了一组不精确切割的产品(短瓣,缺口和缝隙),这些产物通过POLγ通过3'端链的延伸或切除而转化为可韧带的缺口。这取决于POLγ的3'-5'核酸外切酶活性,该酶限制了链置换的活性,并使POLγ通过3'-5'的降解回到了切口。我们还证明了POLγ驱动的链置换足以产生DNA-但不包括RNA-flap的底物,适合在复制过程中进行MGME1裂解和连接。我们的发现对RNA引物去除模型,OriH新生DNA的5'末端加工以及DNA修复具有影响。

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