首页> 外文期刊>Nucleic Acids Research >Enrichment of oligo(dG).oligo(dC)-containing fragments from human genomic DNA by Mg 2+-dependent triplex affinity capture.
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Enrichment of oligo(dG).oligo(dC)-containing fragments from human genomic DNA by Mg 2+-dependent triplex affinity capture.

机译:通过依赖Mg 2+的三链体亲和力捕获从人类基因组DNA富集含oligo(dG).oligo(dC)的片段。

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摘要

Oligo(dG).oligo(dC)- or short poly(dG).poly(dC)-containing fragments were enriched and cloned by means of Mg2+-dependent triplex affinity capture and subsequent cloning procedures. A library constructed after three cycles of enrichment showed that approximately 80% of the clones in the supercoiled form formed a complex with labeled oligonucleotide (dG)34. However, while the rest of the clones retained the ability to form a complex (type I clones), 90.9% failed to form a complex when they were linearized. This group of DNA was abundant in the genomic DNA, although it showed only approximately 3-fold enrichment by one cycle of affinity capture. This group was further classified into two species (types II and III) based on complex formation ability after phenol extraction. Type II clones retained the complex formation ability after treatment, while the human telomere [(TTAGGG)n] and telomere-like [(TGGAA)n] or [(TGGAG)n] sequences belonging to type III clones did not. Serial deletion experiments and the binding assays using oligonucleotides confirmed that the repetitive units containing T(G)nT ( n = 3-5) tracts or (G)n-motifs (n >/= 3) were the sites of complex formation for type II and III clones. On the other hand, type I clones contained poly(dG).poly(dC) tracts at least 10 nt long, and DNase I-footprinting analysis indicated that these tracts were the sites of complex formation.
机译:Oligo(dG).oligo(dC)-或短的poly(dG).poly(dC)含片段被富集并通过Mg2 +依赖的三链体亲和捕获和随后的克隆程序克隆。经过三个富集循环后构建的文库显示,超螺旋形式的克隆中约有80%与标记的寡核苷酸(dG)34形成了复合物。然而,尽管其余克隆保留了形成复合物的能力(I型克隆),但是当线性化它们时,有90.9%的人无法形成复合物。这一组DNA在基因组DNA中很丰富,尽管通过一个亲和力捕获周期仅显示出大约3倍的富集。根据酚提取后的络合物形成能力,该组进一步分为两个种类(II型和III型)。 II型克隆在处理后保留了复杂的形成能力,而属于III型克隆的人端粒[(TTAGGG)n]和端粒状[[TGGAA] n]或[(TGGAG)n]序列则没有。序列缺失实验和使用寡核苷酸的结合试验证实,含有T(G)nT(n = 3-5)片段或(G)n-基序(n> / = 3)的重复单元是该类型复合物的形成位点II和III克隆。另一方面,I型克隆包含至少10 nt长的poly(dG).poly(dC)片段,DNase I足迹分析表明这些片段是复合物形成的位点。

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