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Investigating the Effect of Mono- and Dimeric 360A G-Quadruplex Ligands on Telomere Stability by Single Telomere Length Analysis (STELA)

机译:通过单端粒长度分析(STELA)研究单体和二聚体360A G四联体配体对端粒稳定性的影响

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摘要

Telomeres are nucleoprotein structures that cap and protect the natural ends of chromosomes. Telomeric DNA G-rich strands can form G-quadruplex (or G4) structures. Ligands that bind to and stabilize G4 structures can lead to telomere dysfunctions by displacing shelterin proteins and/or by interfering with the replication of telomeres. We previously reported that two pyridine dicarboxamide G4 ligands, 360A and its dimeric analogue (360A)2A, were able to displace in vitro hRPA (a single-stranded DNA-binding protein of the replication machinery) from telomeric DNA by stabilizing the G4 structures. In this paper, we perform for the first time single telomere length analysis (STELA) to investigate the effect of G4 ligands on telomere length and stability. We used the unique ability of STELA to reveal the full spectrum of telomere lengths at a chromosome terminus in cancer cells treated with 360A and (360A)2A. Upon treatment with these ligands, we readily detected an increase of ultrashort telomeres, whose lengths are significantly shorter than the mean telomere length, and that could not have been detected by other methods.
机译:端粒是核蛋白结构,可覆盖并保护染色体的天然末端。端粒DNA富含G的链可形成G-四链体(或G4)结构。结合并稳定G4结构的配体可通过置换庇护蛋白和/或干扰端粒的复制而导致端粒功能障碍。我们以前报道过,两个吡啶二甲酰胺G4配体360A及其二聚体类似物(360A)2A能够通过稳定G4结构从端粒DNA取代体外hRPA(复制机制的单链DNA结合蛋白)。在本文中,我们首次进行了单端粒长度分析(STELA),以研究G4配体对端粒长度和稳定性的影响。我们利用STELA的独特功能揭示了经360A和(360A)2A处理的癌细胞在染色体末端的端粒全长谱。用这些配体处理后,我们很容易检测到超短端粒的增加,其长度明显短于平均端粒长度,而其他方法则无法检测到。

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