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Time-resolved fluorescence of 2-aminopurine as a probe of base flipping in M.HhaI-DNA complexes

机译:时间分辨的2-氨基嘌呤荧光作为M.HhaI-DNA复合物中碱基翻转的探针

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摘要

DNA base flipping is an important mechanism in molecular enzymology, but its study is limited by the lack of an accessible and reliable diagnostic technique. A series of crystalline complexes of a DNA methyltransferase, M.HhaI, and its cognate DNA, in which a fluorescent nucleobase analogue, 2-aminopurine (AP), occupies defined positions with respect the target flipped base, have been prepared and their structures determined at higher than 2 angstrom resolution. From time-resolved fluorescence measurements of these single crystals, we have established that the fluorescence decay function of AP shows a pronounced, characteristic response to base flipping: the loss of the very short (similar to 100 ps) decay component and the large increase in the amplitude of the long (similar to 10 ns) component. When AP is positioned at sites other than the target site, this response is not seen. Most significantly, we have shown that the same clear response is apparent when M.HhaI complexes with DNA in solution, giving an unambiguous signal of base flipping. Analysis of the AP fluorescence decay function reveals conformational heterogeneity in the DNA-enzyme complexes that cannot be discerned from the present X-ray structures.
机译:DNA碱基翻转是分子酶学中的重要机制,但由于缺乏可访问且可靠的诊断技术,其研究受到了限制。已经制备了一系列DNA甲基转移酶M.HhaI及其同源DNA的晶体复合物,其中荧光核碱基类似物2-氨基嘌呤(AP)相对于目标翻转碱基具有确定的位置,并确定了其结构高于2埃的分辨率。通过对这些单晶进行时间分辨的荧光测量,我们确定了AP的荧光衰减功能对碱基翻转表现出明显的特征响应:非常短的(约100 ps)衰减分量的损失和长(类似于10 ns)分量的幅度。当AP位于目标站点以外的站点时,看不到此响应。最重要的是,我们已经表明,当M.HhaI与溶液中的DNA络合时,同样的清晰反应是显而易见的,从而给出了碱基翻转的明确信号。对AP荧光衰减功能的分析揭示了DNA-酶复合物中的构象异质性,无法从目前的X射线结构中分辨出来。

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