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Real-time observation of DNA repair: 2-aminopurine as a molecular probe

机译:DNA修复的实时观察:2-氨基嘌呤作为分子探针

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Triplex forming oligos (TFOs) that target psoralen photoadducts to specific DNA sequences have generated interest as a potential agent in gene therapy. TFOs also offer an opportunity to study the mechanism of DNA repair in detail. In an effort to understand the mechanism of DNA repair at a specific DNA sequence in real-time, we have designed a plasmid containing a psoralen reaction site adjacent to a TFO binding site corresponding to a sequence within the human interstitial collagenase gene. Two 2-aminopurine residues incorporated into the purine-rich strand of the TFO binding site and located within six nucleotides of the psoralen reaction site serve as molecular probes for excision repair events involving the psoralen photoadducts on that DNA strand. In duplex DNA, the 2-aminopurine fluorescence is quenched. However, upon thermal or formamide-induced denaturation of duplex DNA to single stranded DNA, the 2-aminopurine fluorescence increases by eight fold. These results suggest that monitoring 2-aminopurine fluorescence from plasmids damaged by psoralen TFOs may be a method for measuring excision of single-stranded damaged DNA from the plasmid in cells. A fluorescence-based molecular probe to the plasmid may significantly simplify the real-time observation of DNA repair in both populations of cells as well as single cells.
机译:三螺旋形成寡核苷酸(TFOS),该目标补骨脂photoadducts到特定的DNA序列已经产生了兴趣,如基因治疗的潜在药剂。 TFOS还提供了一个机会来研究DNA修复的详细机制。在努力了解DNA修复中的实时的特定DNA序列的机制,我们设计了含有邻接对应于人类间质胶原酶基因内的序列的TFO结合位点补骨脂素反应位点的质粒。掺入到TFO结合位点的富含嘌呤的链和位于所述补骨脂素反应位点的六个核苷酸内的两个2-氨基嘌呤残基作为涉及对DNA链的补骨脂photoadducts切除修复事件的分子探针。在双链DNA中,2-氨基嘌呤荧光被淬灭。然而,当以单链DNA,双链DNA的热或甲酰胺诱导的变性,通过八倍的2-氨基嘌呤荧光增加。这些结果表明,由补骨脂TFOS损坏质粒监测2-氨基嘌呤荧光可以是用于从细胞中的质粒测量单链DNA损伤的切除的方法。基于荧光的分子探针的质粒可以显著简化DNA修复的实时观察在细胞以及单细胞的两个群体。

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