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Non-Random mtDNA Segregation Patterns Indicate a Metastable Heteroplasmic Segregation Unit in m.3243A>G Cybrid Cells

机译:非随机的mtDNA分离模式表明m.3243A> G杂交细胞中亚稳态的异质分离单元。

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摘要

Many pathogenic mitochondrial DNA mutations are heteroplasmic, with a mixture of mutated and wild-type mtDNA present within individual cells. The severity and extent of the clinical phenotype is largely due to the distribution of mutated molecules between cells in different tissues, but mechanisms underpinning segregation are not fully understood. To facilitate mtDNA segregation studies we developed assays that measure m.3243A>G point mutation loads directly in hundreds of individual cells to determine the mechanisms of segregation over time. In the first study of this size, we observed a number of discrete shifts in cellular heteroplasmy between periods of stable heteroplasmy. The observed patterns could not be parsimoniously explained by random mitotic drift of individual mtDNAs. Instead, a genetically metastable, heteroplasmic mtDNA segregation unit provides the likely explanation, where stable heteroplasmy is maintained through the faithful replication of segregating units with a fixed wild-type/m.3243A>G mutant ratio, and shifts occur through the temporary disruption and re-organization of the segregation units. While the nature of the physical equivalent of the segregation unit remains uncertain, the factors regulating its organization are of major importance for the pathogenesis of mtDNA diseases.
机译:许多致病性线粒体DNA突变是异质的,单个细胞内存在突变和野生型mtDNA的混合物。临床表型的严重程度和程度很大程度上是由于突变分子在不同组织中的细胞之间的分布所致,但是支撑分离的机制尚不完全清楚。为促进mtDNA分离研究,我们开发了可直接在数百个单个细胞中测量m.3243A> G点突变负荷的测定方法,以确定随时间推移的分离机制。在这种大小的第一个研究中,我们观察到细胞质异质性在稳定异质性期间之间发生了许多离散变化。单个mtDNA的随机有丝分裂漂移无法简约地解释观察到的模式。相反,遗传上亚稳态的异质mtDNA分离单元提供了可能的解释,其中通过忠实复制具有固定野生型/m.3243A>G突变体比率的分离单元来维持稳定的异质性,并且通过暂时破坏和转移而发生转移。重组隔离单位。尽管分离单位的物理等同物的性质仍然不确定,但调节其组织的因素对于mtDNA疾病的发病机理至关重要。

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