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通过三链螺旋形成实现双链螺旋DNA的序列特异性切割。

Sequence-specific cleavage of double helical DNA by triple helix formation.

作者信息

Moser H E, Dervan P B

机构信息

Division of Chemistry and Chemical Engineering, California Institute of Technology, Pasadena 91125.

出版信息

Science. 1987 Oct 30;238(4827):645-50. doi: 10.1126/science.3118463.

Abstract

Homopyrimidine oligodeoxyribonucleotides with EDTA-Fe attached at a single position bind the corresponding homopyrimidine-homopurine tracts within large double-stranded DNA by triple helix formation and cleave at that site. Oligonucleotides with EDTA.Fe at the 5' end cause a sequence specific double strand break. The location and asymmetry of the cleavage pattern reveal that the homopyrimidine-EDTA probes bind in the major groove parallel to the homopurine strand of Watson-Crick double helical DNA. The sequence-specific recognition of double helical DNA by homopyrimidine probes is sensitive to single base mismatches. Homopyrimidine probes equipped with DNA cleaving moieties could be useful tools for mapping chromosomes.

摘要

在单个位置连接有乙二胺四乙酸铁(EDTA-Fe)的同嘧啶寡聚脱氧核糖核苷酸通过三链螺旋的形成与大的双链DNA内相应的同嘧啶-同嘌呤片段结合,并在该位点切割。5'端带有EDTA.Fe的寡核苷酸会导致序列特异性双链断裂。切割模式的位置和不对称性表明,同嘧啶-EDTA探针在与沃森-克里克双螺旋DNA的同嘌呤链平行的大沟中结合。同嘧啶探针对双链DNA的序列特异性识别对单碱基错配敏感。配备有DNA切割部分的同嘧啶探针可能是用于染色体图谱绘制的有用工具。

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