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DNA探针与溶液中RNA的定量杂交动力学,随后进行扩散荧光相关分析。

Quantitative hybridization kinetics of DNA probes to RNA in solution followed by diffusional fluorescence correlation analysis.

作者信息

Schwille P, Oehlenschläger F, Walter N G

机构信息

Max-Planck-Institute for Biophysical Chemistry, Department of Biochemical Kinetics, Göttingen, Germany.

出版信息

Biochemistry. 1996 Aug 6;35(31):10182-93. doi: 10.1021/bi960517g.

DOI:10.1021/bi960517g
PMID:8756483
Abstract

Binding kinetics in solution of six N,N,N',N'-tetramethyl-5-carboxyrhodamine-labeled oligodeoxyribonucleotide probes to a 101mer target RNA comprising the primer binding site for HIV-1 reverse transcriptase were characterized using fluorescence correlation spectroscopy (FCS). FCS allows a sensitive, non-radioactive real time observation of hybridization of probes to the RNA target in the buffer of choice without separation of free and bound probe. The binding process could directly be monitored by the change in translational diffusion time of the 17mer to 37mer DNA probe upon specific hybridization with the larger RNA target. The characteristic diffusion time through a laser-illuminated open volume element with 0.5 micron in diameter increased from 0.13-0.2 ms (free) to 0.37-0.50 ms (bound), depending on the probe. Hybridization was approximated by biphasic irreversible second-order reaction kinetics, yielding first-phase association rate constants between 3 x 10(4) and 1.5 x 10(6) M-1 s-1 for the different probes. These varying initial rates reflected the secondary structures of probes and target sites, being consistent with a hypothetical binding pathway starting from loop-loop interactions in a kissing complex, and completion of hybridization requiring an additional interaction involving single-stranded regions of both probe and target. FCS thus permits rapid screening for suitable antisense nucleic acids directed against an important target like HIV-1 RNA with low consumption of probes and target.

摘要

使用荧光相关光谱法(FCS)对六种N,N,N',N'-四甲基-5-羧基罗丹明标记的寡脱氧核糖核苷酸探针与包含HIV-1逆转录酶引物结合位点的101聚体靶RNA在溶液中的结合动力学进行了表征。FCS能够在不分离游离探针和结合探针的情况下,在所选缓冲液中对探针与RNA靶标的杂交进行灵敏、非放射性的实时观察。通过17聚体至37聚体DNA探针与较大RNA靶标特异性杂交后平移扩散时间的变化,可以直接监测结合过程。根据探针的不同,通过直径为0.5微米的激光照射开放体积元件的特征扩散时间从0.13 - 0.2毫秒(游离)增加到0.37 - 0.50毫秒(结合)。杂交过程近似为双相不可逆二级反应动力学,不同探针的第一阶段缔合速率常数在3×10⁴至1.5×10⁶ M⁻¹ s⁻¹之间。这些不同的初始速率反映了探针和靶位点的二级结构,这与从亲吻复合物中的环 - 环相互作用开始的假设结合途径一致,并且杂交的完成需要涉及探针和靶标的单链区域的额外相互作用。因此,FCS允许以低探针和靶标消耗快速筛选针对HIV-1 RNA等重要靶标的合适反义核酸。

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