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DeltaDelta - [{Ru(phen)₂}₂(μ - dppm)]⁴⁺(dppm 为 4,6 - 双(2 - 吡啶基)嘧啶;phen 为 1,10 - 菲咯啉)在 DNA 结合时在三碱基凸起位点的选择性 。

Selectivity at a three-base bulge site in the DNA binding of DeltaDelta-[{Ru(phen)2} 2(mu-dppm)]4+ [dppm is 4,6-bis(2-pyridyl)pyrimidine; phen is 1,10-phenanthroline].

作者信息

Morgan Joy L, Buck Damian P, Turley Adam G, Collins J Grant, Keene F Richard

机构信息

Department of Chemistry, School of Pharmacy & Molecular Sciences, James Cook University, Townsville, QLD, 4811, Australia.

出版信息

J Biol Inorg Chem. 2006 Oct;11(7):824-34. doi: 10.1007/s00775-006-0130-9. Epub 2006 Jun 28.

Abstract

The binding of the stereoisomers of [{Ru(phen)2}2(mu-bpm)]4+, [{Ru(phen)2}2(mu-dppm)]4+ and [{Ru(phen)2}2(mu-bb)]4+ {phen is 1,10-phenanthroline; bpm is 2,2'-bipyrimidine, dppm is 4,6-bis(2-pyridyl)pyrimidine, bb is 1,2-bis[4-(4'-methyl-2,2'-bipyridyl)]ethane} to an oligonucleotide duplex [d(GCATCGAAAGCTACG).d(CGTAGCCGATGC)] containing a three-base bulge has been studied using a fluorescence intercalator displacement assay. Of the dinuclear ruthenium complexes, the dppm-linked species showed the strongest binding to the oligonucleotide, with the DeltaDelta isomer binding slightly more strongly than the meso isomer and the LambdaLambda isomer exhibiting the weakest binding. In order to determine whether the DeltaDelta-[{Ru(phen)2}2(mu-dppm)]4+ metal complex specifically bound at the three-base bulge site, a 1H NMR study of the binding of the metal complex to the oligonucleotide duplex d(GCATCGAAAGCTACG)*d(CGTAGCCGATGC) was carried out. Although a detailed picture of the metal complex-oligonucleotide association could not be determined from the NMR results owing to the broadening of the resonances from the metal complex and nucleotide residues at the bulge site, the NMR results do indicate that the metal complex specifically binds at the three-base bulge site. The combined results of this study suggest that the dppm-bridged dinuclear ruthenium complexes have considerable potential as probes for the unusual secondary structure obtained by the insertion of a three-base bulge within duplex DNA.

摘要

使用荧光嵌入剂置换分析法研究了[{Ru(phen)2}2(μ-bpm)]4+、[{Ru(phen)2}2(μ-dppm)]4+和[{Ru(phen)2}2(μ-bb)]4+(phen为1,10-菲咯啉;bpm为2,2'-联嘧啶,dppm为4,6-双(2-吡啶基)嘧啶,bb为1,2-双[4-(4'-甲基-2,2'-联吡啶)]乙烷)的立体异构体与含有三碱基凸起的寡核苷酸双链体[d(GCATCGAAAGCTACG).d(CGTAGCCGATGC)]的结合情况。在双核钌配合物中,与dppm相连的物种对寡核苷酸的结合最强,其中ΔΔ异构体的结合略强于内消旋异构体,而ΛΛ异构体的结合最弱。为了确定ΔΔ-[{Ru(phen)2}2(μ-dppm)]4+金属配合物是否特异性结合在三碱基凸起位点上,对该金属配合物与寡核苷酸双链体d(GCATCGAAAGCTACG)*d(CGTAGCCGATGC)的结合进行了1H NMR研究。尽管由于凸起位点处金属配合物和核苷酸残基的共振变宽,无法从NMR结果中确定金属配合物-寡核苷酸缔合的详细情况,但NMR结果确实表明该金属配合物特异性结合在三碱基凸起位点上。本研究的综合结果表明,dppm桥连的双核钌配合物作为探测双链DNA中插入三碱基凸起所获得的异常二级结构的探针具有相当大的潜力。

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