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Excitonic Heterodimer Formation in an HIV-1 Oligonucleotide Labeled with a Donor-Acceptor Pair Used for Fluorescence Resonance Energy Transfer

机译:激子异二聚体形成的HIV-1寡核苷酸标记的供体-受体对用于荧光共振能量转移。

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摘要

In this study, we investigated the absorbance and fluorescence properties of cTAR, the complementary DNA sequence of the transactivation response element of the HIV-1 genome, doubly end-labeled by different dyes, 5(and 6)-carboxyfluorescein (Fl) and 5(and 6)-carboxytetramethylrhodamine (TMR), frequently used in fluorescence resonance energy transfer (FRET) studies. This oligonucleotide forms a stable stem-loop structure. The absorption spectrum of this species clearly differed from that of a doubly labeled cTAR derivative in which the terminal part of the stem is melted and from an equimolecular mixture of singly labeled species. Moreover, no significant TMR fluorescence change accompanies the dramatic Fl intensity increase when the doubly labeled native cTAR was melted by temperature or annealed with its complementary sequence. Both elements suggest the formation of an H-type ground-state heterodimer between Fl and TMR that may be described by the molecular exciton model. Moreover, time-resolved fluorescence further suggests that the nonfluorescent heterodimer is in equilibrium with a small population of partially melted species showing FRET. Based on the spectral shifts associated with heterodimer formation, an interchromophore distance of 7.7 Å was calculated. Both the excitonic signal and the Fl fluorescence were used as sensitive tools to monitor the temperature-mediated and HIV nucleocapsid protein-mediated annealing of cTAR with its complementary sequence.
机译:在这项研究中,我们研究了cTAR的吸收和荧光特性,HIV-1基因组反式激活元件的互补DNA序列,被不同染料,5(和6)-羧基荧光素(F1)和5双重标记。 (和6)-羧基四甲基罗丹明(TMR),常用于荧光共振能量转移(FRET)研究中。该寡核苷酸形成稳定的茎环结构。该物质的吸收光谱与双标记的cTAR衍生物的吸收光谱明显不同,双核cTAR衍生物的茎的末端部分被熔化,并且与单标记的物质的等分子混合物不同。而且,当双标记的天然cTAR通过温度融化或与其互补序列退火时,没有显着的TMR荧光变化伴随F1强度的急剧增加。两种元素都暗示在F1和TMR之间形成H型基态异二聚体,这可由分子激子模型描述。此外,时间分辨的荧光进一步表明,非荧光异二聚体与少量的部分熔融物种处于平衡状态,表现出FRET。基于与异二聚体形成相关的光谱位移,计算出发色团间距离为7.7。激子信号和F1荧光均被用作敏感工具,以监测温度介导的和cHIV核衣壳蛋白介导的cTAR及其互补序列的退火。

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