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Highly specific and sensitive method for measuring nucleotide excision repair kinetics of ultraviolet photoproducts in human cells

机译:测量人体细胞中紫外线光产物核苷酸切除修复动力学的高特异性和灵敏方法

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摘要

The nucleotide excision repair pathway removes ultraviolet (UV) photoproducts from the human genome in the form of short oligonucleotides ~30 nt in length. Because there are limitations to many of the currently available methods for investigating UV photoproduct repair in vivo, we developed a convenient non-radioisotopic method to directly detect DNA excision repair events in human cells. The approach involves extraction of oligonucleotides from UV-irradiated cells, DNA end-labeling with biotin and streptavidin-mediated chemiluminescent detection of the excised UV photoproduct-containing oligonucleotides that are released from the genome during excision repair. Our novel approach is robust, with essentially no signal in the absence of UV or a functional excision repair system. Furthermore, our non-radioisotopic methodology allows for the sensitive detection of excision products within minutes following UV irradiation and does not require additional enrichment steps such as immunoprecipitation. Finally, this technique allows for quantitative measurements of excision repair in human cells. We suggest that the new techniques presented here will be a useful and powerful approach for studying the mechanism of human nucleotide excision repair in vivo.
机译:核苷酸切除修复途径以长度约30 nt的短寡核苷酸形式从人类基因组中去除了紫外线(UV)光产物。由于目前许多用于研究体内UV光产物修复的方法均存在局限性,因此我们开发了一种方便的非放射性同位素方法来直接检测人细胞中的DNA切除修复事件。该方法涉及从受紫外线照射的细胞中提取寡核苷酸,用生物素进行DNA末端标记以及链霉亲和素介导的化学切除检测,以在切除修复过程中从基因组中释放出已切除的含紫外线光产物的寡核苷酸。我们的新方法功能强大,在没有紫外线或功能性切除修复系统的情况下基本没有信号。此外,我们的非放射性同位素方法可在紫外线照射后数分钟内灵敏地检测出切除产物,并且不需要其他富集步骤,例如免疫沉淀。最后,该技术允许定量测量人体细胞中的切除修复。我们建议这里介绍的新技术将是一种有用的和强大的方法,用于研究体内人类核苷酸切除修复的机制。

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