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在三链体 - 双链体连接处的位点特异性嵌入会引发一种构象变化,这种变化可通过对焦碳酸二乙酯的超敏反应检测到。

Site-specific intercalation at the triplex-duplex junction induces a conformational change which is detectable by hypersensitivity to diethylpyrocarbonate.

作者信息

Collier D A, Mergny J L, Thuong N T, Helene C

机构信息

Laboratoire de Biophysique, Museum National d'Histoire Naturelle, Inserm U201, CNRS UA 481, Paris, France.

出版信息

Nucleic Acids Res. 1991 Aug 11;19(15):4219-24. doi: 10.1093/nar/19.15.4219.

Abstract

Using site-specific intercalation directed by intermolecular triplex formation, the conformation of an intercalation site in DNA was examined by footprinting with the purine-specific (A much greater than G) reagent diethylpyrocarbonate. Site specific intercalation was achieved by covalently linking an intercalator to the 5' end of a homopyrimidine oligodeoxynucleotide, which bound to a homopurinehomopyrimidine stretch in a recombinant plasmid via intermolecular triplex formation. This directs intercalation to a single site in 3kb of DNA at the 5' triplex-duplex junction. Footprinting with diethylpyrocarbonate and dimethylsulphate revealed strong protection from modification of adenine residues within the triple-helix in concordance with their Hoogsteen pairing with the third strand, and a strong hypersensitivity to diethylpyrocarbonate at the first adenine of the duplex. This result indicates that intercalation at this site induces a conformational change at the 5' triplex-duplex junction. Furthermore, the same diethlypyrocarbonate hypersensitivity was observed with an unmodified triple-strand forming oligonucleotide and a range of intercalating molecules present in solution. Thus the 5' triplex-duplex junction is a strong binding site for some intercalating molecules and the junction undergoes a conformational change which is sensitive to diethylpyrocarbonate upon insertion of the planar aromatic chromophore. This conformational change can be used to direct a single-strand cut in duplex DNA to a defined site.

摘要

利用由分子间三链体形成引导的位点特异性嵌入,通过用嘌呤特异性(A远大于G)试剂焦碳酸二乙酯进行足迹分析,研究了DNA中嵌入位点的构象。通过将嵌入剂共价连接到同嘧啶寡脱氧核苷酸的5'端来实现位点特异性嵌入,该寡脱氧核苷酸通过分子间三链体形成与重组质粒中的同嘌呤-同嘧啶片段结合。这将嵌入引导至3kb DNA中5'三链体-双链体交界处的单个位点。用焦碳酸二乙酯和硫酸二甲酯进行足迹分析表明,与它们与第三条链的Hoogsteen配对一致,三链体内的腺嘌呤残基受到强烈的保护而不被修饰,并且双链体的第一个腺嘌呤对焦碳酸二乙酯有强烈的超敏感性。这一结果表明,该位点的嵌入在5'三链体-双链体交界处诱导了构象变化。此外,用未修饰的三链体形成寡核苷酸和溶液中存在的一系列嵌入分子观察到相同的焦碳酸二乙酯超敏感性。因此,5'三链体-双链体交界处是一些嵌入分子的强结合位点,并且在平面芳香发色团插入时,该交界处会发生对焦碳酸二乙酯敏感的构象变化。这种构象变化可用于将双链DNA中的单链切割引导至特定位点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2197/328565/9d7cff601dbd/nar00095-0178-a.jpg

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