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人类细胞中的异源线粒体DNA重组

Heterologous mitochondrial DNA recombination in human cells.

作者信息

D'Aurelio Marilena, Gajewski Carl D, Lin Michael T, Mauck William M, Shao Leon Z, Lenaz Giorgio, Moraes Carlos T, Manfredi Giovanni

机构信息

Department of Neurology and Neuroscience, Weill Medical College of Cornell University, New York, NY, USA.

出版信息

Hum Mol Genet. 2004 Dec 15;13(24):3171-9. doi: 10.1093/hmg/ddh326. Epub 2004 Oct 20.

Abstract

Inter-molecular heterologous mitochondrial DNA (mtDNA) recombination is known to occur in yeast and plants. Nevertheless, its occurrence in human cells is still controversial. To address this issue we have fused two human cytoplasmic hybrid cell lines, each containing a distinct pathogenic mtDNA mutation and specific sets of genetic markers. In this hybrid model, we found direct evidence of recombination between these two mtDNA haplotypes. Recombinant mtDNA molecules in the hybrid cells were identified using three independent experimental approaches. First, recombinant molecules containing genetic markers from both parental alleles were demonstrated with restriction fragment length polymorphism of polymerase chain reaction products, by measuring the relative frequencies of each marker. Second, fragments of recombinant mtDNA were cloned and sequenced to identify the regions involved in the recombination events. Finally, recombinant molecules were demonstrated directly by Southern blot using appropriate combinations of polymorphic restriction sites and probes. This combined approach confirmed the existence of heterogeneous species of recombinant mtDNA molecules in the hybrid cells. These findings have important implications for mtDNA-related diseases, the interpretation of human evolution and population genetics and forensic analyses based on mtDNA genotyping.

摘要

分子间异源线粒体DNA(mtDNA)重组在酵母和植物中已被证实会发生。然而,其在人类细胞中的发生仍存在争议。为解决这一问题,我们将两个人类细胞质杂交细胞系进行了融合,每个细胞系都含有独特的致病性mtDNA突变和特定的遗传标记集。在这个杂交模型中,我们发现了这两种mtDNA单倍型之间重组的直接证据。杂交细胞中的重组mtDNA分子通过三种独立的实验方法得以鉴定。首先,通过测量每个标记的相对频率,利用聚合酶链反应产物的限制性片段长度多态性,证明了含有来自两个亲本等位基因遗传标记的重组分子。其次,克隆并测序重组mtDNA的片段,以确定参与重组事件的区域。最后,使用多态性限制性位点和探针的适当组合,通过Southern印迹直接证明重组分子。这种综合方法证实了杂交细胞中存在重组mtDNA分子的异质物种。这些发现对于与mtDNA相关的疾病、人类进化和群体遗传学的解释以及基于mtDNA基因分型的法医分析具有重要意义。

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