Malinge J M, Schwartz A, Leng M
Nucleic Acids Res. 1987 Feb 25;15(4):1779-97. doi: 10.1093/nar/15.4.1779.
The purpose of this study was to characterize the ternary complexes formed in the reaction of cis-diamminedichloroplatinum (II) (cis-DDP) and nucleic acids, in the presence of the intercalating compound ethidium bromide (EtBr). In these ternary complexes, some EtBr is tightly bound to the nucleic acids. Tight binding is defined by resistance to extraction with butanol, assayed by filtration at acid pH or thin layer chromatography at basic pH. These ternary complexes are formed with double stranded but not with single stranded nucleic acids. They are not formed if cis-DDP is replaced by transdiamminedichloroplatinum(II). The amount of tightly bound EtBr depends upon the sequence of the nucleic acid, being larger with poly (dG-dC).poly(dG-dC) than with poly(dG).poly(dC). Spectroscopic results support the hypothesis that the tight binding of the dye is due to the formation of a bidentate adduct (guanine-EtBr)cis-platin. The visible spectrum of the ternary complexes is blue-shifted as compared to that of EtBr intercalated between the base pairs of unplatinated DNA and it depends upon the conformation of the ternary complex. The fluorescence quantum yield of the ternary complexes is lower than that of free EtBr in water. Tightly bound EtBr stabilizes strongly the B form versus the Z form of the ternary complex poly(dG-dC)-Pt-EtBr and slows down the transition from the B form towards the Z form. The sequence specificity of cis-DDP binding to a DNA restriction fragment in the absence or presence of EtBr is mapped by means of the 3'----5' exonuclease activity of T4 DNA polymerase. In the absence of the dye, all the d(GpG) sites and all the d(ApG) sites but one in the sequence d(TpGpApGpC) are platinated. The d(GpA) sites are not platinated. In the presence of EtBr, some new sites are detected. These results might help to explain the synergism for drugs used in combination with cis-DDP and in the design of new chemotherapeutic agents.
本研究的目的是表征在嵌入化合物溴化乙锭(EtBr)存在下,顺二氯二氨合铂(II)(顺铂)与核酸反应形成的三元复合物。在这些三元复合物中,一些EtBr与核酸紧密结合。紧密结合通过对用丁醇萃取的抗性来定义,通过在酸性pH下过滤或在碱性pH下进行薄层色谱分析。这些三元复合物由双链而非单链核酸形成。如果用反式二氯二氨合铂(II)代替顺铂,则不会形成它们。紧密结合的EtBr的量取决于核酸的序列,聚(dG-dC)·聚(dG-dC)比聚(dG)·聚(dC)中的量更大。光谱结果支持这样的假设,即染料的紧密结合是由于形成了双齿加合物(鸟嘌呤-EtBr)顺铂。与嵌入未铂化DNA碱基对之间的EtBr相比,三元复合物的可见光谱发生蓝移,并且它取决于三元复合物的构象。三元复合物的荧光量子产率低于水中游离EtBr的荧光量子产率。紧密结合的EtBr相对于三元复合物聚(dG-dC)-Pt-EtBr的Z型强烈稳定B型,并减缓从B型向Z型的转变。通过T4 DNA聚合酶的3'→5'核酸外切酶活性,绘制了在不存在或存在EtBr的情况下顺铂与DNA限制片段结合的序列特异性图谱。在没有染料的情况下,序列d(TpGpApGpC)中的所有d(GpG)位点和除一个之外的所有d(ApG)位点都被铂化。d(GpA)位点未被铂化。在存在EtBr的情况下,检测到一些新位点。这些结果可能有助于解释与顺铂联合使用的药物的协同作用以及新化疗药物的设计。
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