Long-run real-time PCR analysis of repetitive nuclear elements as a novel tool for DNA damage quantification in single cells: an approach validated on mouse oocytes and fibroblasts

被引:2
作者
Kotarska, Katarzyna [1 ]
Gasior, Lukasz [2 ]
Rudnicka, Joanna [3 ,4 ]
Polanski, Zbigniew [1 ]
机构
[1] Jagiellonian Univ, Inst Zool & Biomed Res, Lab Genet & Evolut, Krakow, Poland
[2] Polish Acad Sci, Inst Pharmacol, Dept Neurobiol, Lab Neurobiol Trace Elements, Krakow, Poland
[3] Jagiellonian Univ, Malopolska Ctr Biotechnol, Krakow, Poland
[4] Jagiellonian Univ, Doctoral Sch Exact & Nat Sci, Krakow, Poland
关键词
DNA lesions; L1; elements; LORD-Q method; Single-cell genome; qPCR; DOUBLE-STRAND BREAKS; MITOCHONDRIAL-DNA; REPAIR; EMBRYOS; MARKER;
D O I
10.1007/s13353-023-00817-0
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Since DNA damage is of great importance in various biological processes, its rate is frequently assessed both in research studies and in medical diagnostics. The most precise methods of quantifying DNA damage are based on real-time PCR. However, in the conventional version, they require a large amount of genetic material and therefore their usefulness is limited to multicellular samples. Here, we present a novel approach to long-run real-time PCR-based DNA-damage quantification (L1-LORD-Q), which consists in amplification of long interspersed nuclear elements (L1) and allows for analysis of single-cell genomes. The L1-LORD-Q was compared with alternative methods of measuring DNA breaks (Bioanalyzer system, gamma-H2AX foci staining), which confirmed its accuracy. Furthermore, it was demonstrated that the L1-LORD-Q is sensitive enough to distinguish between different levels of UV-induced DNA damage. The method was validated on mouse oocytes and fibroblasts, but the general idea is universal and can be applied to various types of cells and species.
引用
收藏
页码:181 / 190
页数:10
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