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将患有神经病变、共济失调和色素性视网膜炎(NARP)的患者的异质性线粒体DNA(mtDNA)导入两个人类ρ0细胞系,要么与NARP突变型mtDNA的选择和维持有关,要么与mtDNA维持失败有关。

Introduction of heteroplasmic mitochondrial DNA (mtDNA) from a patient with NARP into two human rho degrees cell lines is associated either with selection and maintenance of NARP mutant mtDNA or failure to maintain mtDNA.

作者信息

Vergani L, Rossi R, Brierley C H, Hanna M, Holt I J

机构信息

Department of Molecular Pathology, University of Dundee, UK.

出版信息

Hum Mol Genet. 1999 Sep;8(9):1751-5. doi: 10.1093/hmg/8.9.1751.

Abstract

Mitochondria from a patient heteroplasmic at nucleo-tide position 8993 of mitochondrial DNA (mtDNA) were introduced into two human tumour cell lines lacking mtDNA. The donor mitochondria contained between 85 and 95% 8993G:C mtDNA. All detectable mtDNA in the mitochondrially transformed cells contained the pathological 8993G:C mutation 3 months after transformation. These results suggest that 8993G:C mtDNA had a selective advantage over 8993T:A mtDNA in both lung carcinoma and osteo-sarcoma cell backgrounds. In contrast, two other presumed pathological mtDNA variants were lost in favour of 'wild-type' mtDNA molecules in the same lung carcinoma cell background. Taken together, these findings suggest that the transmission bias of mtDNA variants is dependent upon a combination of nuclear background and mtDNA genotype. A second phenomenon observed was a marked decrease in the growth rate of many putative transformed cell lines after 6 weeks of culturing in selective medium, and in these cell lines mtDNA was not readily detectable by Southern blotting. Restriction endonuclease analysis and sequencing of amplified mtDNA demonstrated that the slow growing cells contained little or no mtDNA. It is concluded that these cells represented transient mitochondrial transformants.

摘要

将来自线粒体DNA(mtDNA)核苷酸位置8993处存在异质性的患者的线粒体导入两个缺乏mtDNA的人类肿瘤细胞系。供体线粒体含有85%至95%的8993G:C型mtDNA。线粒体转化细胞中所有可检测到的mtDNA在转化3个月后都含有病理性的8993G:C突变。这些结果表明,在肺癌和骨肉瘤细胞背景中,8993G:C型mtDNA相对于8993T:A型mtDNA具有选择性优势。相比之下,在相同的肺癌细胞背景中,另外两个推测的病理性mtDNA变体被淘汰,有利于“野生型”mtDNA分子。综上所述,这些发现表明mtDNA变体的传递偏差取决于核背景和mtDNA基因型的组合。观察到的第二个现象是,在选择性培养基中培养6周后,许多假定的转化细胞系的生长速率显著下降,并且在这些细胞系中,通过Southern印迹法不易检测到mtDNA。对扩增的mtDNA进行限制性内切酶分析和测序表明,生长缓慢的细胞几乎不含或不含mtDNA。得出的结论是,这些细胞代表瞬时线粒体转化体。

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