双核钌（II）配合物作为RNA凸起位点的潜在探针。

Spillane Caitriona B, Smith Jayden A, Buck Damian P, Collins J Grant, Keene F Richard

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

Dalton Trans. 2007 Dec 7(45):5290-6. doi: 10.1039/b712065f.

1H NMR spectroscopy and molecular modelling have been used to investigate the binding of the DeltaDelta-and LambdaLambda-enantiomers of the dinuclear ruthenium(II) complex [[Ru(Me2bpy)2]2(mu-bpm)]4+ [Me2bpy = 4,4'-dimethyl-2,2'-bipyridine; bpm = 2,2'-bipyrimidine] to an RNA tridecanucleotide duplex containing a single-base bulge [r(CCGAGAAUUCCGG)2]], and the corresponding control dodecanucleotide [r(CCGGAAUUCCGG)2]. Both enantiomers bound the control RNA sequence weakly. From upfield shifts of the metal complex H3 and H3' protons throughout the titration of the control dodecanucleotide with DeltaDelta-[[Ru(Me2bpy)2]2(mu-bpm)]4+, a binding constant of 1 x 10(3) M(-1) was determined. In NOESY spectra of the control sequence with added DeltaDelta-[[Ru(Me2bpy)2]2(mu-bpm)]4+, NOEs were only observed to protons from the terminal base-pair residues. No significant changes in chemical shift were observed for either the metal complex or RNA protons upon addition of the LambdaLambda-enantiomer to the control dodecanucleotide. The DeltaDelta-[[Ru(Me2bpy)2]2(mu-bpm)]4+ complex bound the bulge-containing RNA with a significantly greater affinity (6 x 10(4) M(-1)) than the non-bulge control RNA duplex. Competition binding experiments indicated that the LambdaLambda-isomer bound the tridecanucleotide with similar affinity to the DeltaDelta-enantiomer. Addition of DeltaDelta-[[Ru(Me2bpy)2]2(mu-bpm)]4+ to the bulge-containing tridecanucleotide induced selective changes in chemical shift for the base H8 and sugar H1' resonances from the adenine bulge residue, and resonances from nucleotide residues adjacent to the bulge site. Intermolecular NOEs observed in NOESY spectra of the tridecanucleotide with added DeltaDelta-[[Ru(Me2bpy)2]2(mu-bpm)]4+ confirmed the selective binding of the ruthenium complex at the bulge site. Preliminary binding models, consistent with the NMR data, showed that the ruthenium complex could effectively associate in the RNA minor groove at the bulge site.

1H核磁共振光谱法和分子建模已被用于研究双核钌（II）配合物[[Ru(Me2bpy)2]2(μ-bpm)]4+ [Me2bpy = 4,4'-二甲基-2,2'-联吡啶；bpm = 2,2'-联嘧啶]的DeltaDelta-和LambdaLambda-对映体与含有单碱基凸起的RNA十三聚体双链体[r(CCGAGAAUUCCGG)2]以及相应的对照十二聚体[r(CCGGAAUUCCGG)2]的结合情况。两种对映体与对照RNA序列的结合都很弱。在用DeltaDelta-[[Ru(Me2bpy)2]2(μ-bpm)]4+滴定对照十二聚体的整个过程中，通过金属配合物H3和H3'质子的高场位移，测定出结合常数为1×10(3) M(-1)。在添加了DeltaDelta-[[Ru(Me2bpy)2]2(μ-bpm)]4+的对照序列的NOESY光谱中，只观察到与末端碱基对残基质子的核Overhauser效应（NOE）。向对照十二聚体中添加LambdaLambda-对映体后，无论是金属配合物还是RNA质子的化学位移都没有观察到显著变化。DeltaDelta-[[Ru(Me2bpy)2]2(μ-bpm)]4+配合物与含有凸起的RNA的结合亲和力（6×10(4) M(-1)）明显高于不含凸起的对照RNA双链体。竞争结合实验表明，LambdaLambda-异构体与十三聚体的结合亲和力与DeltaDelta-对映体相似。向含有凸起的十三聚体中添加DeltaDelta-[[Ru(Me2bpy)2]2(μ-bpm)]4+会导致来自腺嘌呤凸起残基的碱基H8和糖H1'共振以及与凸起位点相邻的核苷酸残基共振的化学位移发生选择性变化。在添加了DeltaDelta-[[Ru(Me2bpy)2]2(μ-bpm)]4+的十三聚体的NOESY光谱中观察到的分子间NOE证实了钌配合物在凸起位点的选择性结合。与NMR数据一致的初步结合模型表明，钌配合物可以在RNA小沟中的凸起位点有效缔合。