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Interaction of minor groove binding ligands with long AT tracts

机译:小沟结合配体与长AT束的相互作用

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We have used quantitative DNase I footprinting to examine the ability of distamycin and Hoechst 33258 to discriminate between different arrangements of AT residues, using synthetic DNA fragments containing multiple blocks of (A/T)6or (A/T)10in identical sequence environments. Previous studies have shown that these ligands bind less well to (A/T)4sites containing TpA steps. We find that in (A/T)6tracts distamycin shows little discrimination between the various sites, binding approximately 2-fold stronger to TAATTA than (TA)3, T3A3and GAATTC. In contrast, Hoechst 33258 binds approximately 20-fold more tightly to GAATTC and TAATTA than T3A3and (TA)3. Hydroxyl radical footprinting reveals that both ligands bind in similar locations at the centre of each AT tract. At (A/T)10sites distamycin binds with similar affinity to T5A5, (TA)5and AATT, though bands in the centre of (TA)5are protected at approximately 50-fold lower concentration than those towards the edges. Hoechst 33258 shows a similar pattern of preference, with strong binding to AATT, T5A5and the centre of (TA)5. Hydroxyl radical footprinting reveals that at low concentrations both ligands bind at the centre of (TA)5and A5T5, while at higher concentrations ligand molecules bind to each end of the (A/T)10tracts. At T5A5two ligand molecules bind at either end of the site, even at the lowest ligand concentration, consistent with the suggestion that these compounds avoid the TpA step. Similar DNase I footprinting experiments with a DNA fragment containing T n (n = 3-6) tracts reveals that both ligands bind in the order T3< T4 T5 = T6.
机译:我们已经使用定量DNase I足迹技术,通过在相同序列环境中使用包含多个(A / T)6或(A / T)10嵌段的合成DNA片段,检查了双霉素和Hoechst 33258区分AT残基不同排列的能力。先前的研究表明,这些配体与包含TpA步骤的(A / T)4位点的结合较弱。我们发现,在(A / T)6分中,地他霉素在各个位点之间几乎没有区别,与(TA)3,T3A3和GAATTC的结合强度约为TAATTA的2倍。相反,与T3A3和(TA)3相比,Hoechst 33258与GAATTC和TAATTA的结合强度大约高20倍。羟基自由基足迹揭示了两个配体在每个AT区域中心的相似位置结合。在(A / T)10位处,间他霉素与T5A5,(TA)5和AATT的亲和力相似,尽管(TA)5中心的条带受保护的浓度比向边缘的条带低约50倍。 Hoechst 33258表现出相似的偏好模式,与AATT,T5A5和(TA)5的中心紧密结合。羟基自由基足迹表明,在低浓度下,两个配体都在(TA)5和A5T5的中心结合,而在较高浓度下,配体分子则在(A / T)10链的每个末端结合。在T5A5处,两个配体分子甚至在最低配体浓度下都在该位点的任一端结合,这与这些化合物避免TpA步骤的建议相符。用含有Tn(n = 3-6)片段的DNA片段进行的类似DNase I足迹实验表明,两个配体的结合顺序为T3

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