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非修饰和双吡啶修饰的 PNA 双链体的晶体结构。

The crystal structure of non-modified and bipyridine-modified PNA duplexes.

机构信息

Department of Structural Biology, University of Pittsburgh Medical School, Pittsburgh, PA 15260, USA.

出版信息

Chemistry. 2010 Oct 18;16(39):11867-75. doi: 10.1002/chem.201000392.

Abstract

Peptide nucleic acid (PNA) is a synthetic analogue of DNA that commonly has an N-aminoethyl glycine backbone. The crystal structures of two PNA duplexes, one containing eight standard nucleobase pairs (GGCATGCC)(2), and the other containing the same nucleobase pairs and a central pair of bipyridine ligands, have been solved with a resolution of 1.22 and 1.10 Å, respectively. The non-modified PNA duplex adopts a P-type helical structure similar to that of previously characterized PNAs. The atomic-level resolution of the structures allowed us to observe for the first time specific modes of interaction between the terminal lysines of the PNA and the backbone and the nucleobases situated in the vicinity of the lysines, which are considered an important factor in the induction of a preferred handedness in PNA duplexes. Our results support the notion that whereas PNA typically adopts a P-type helical structure, its flexibility is relatively high. For example, the base-pair rise in the bipyridine-containing PNA is the largest measured to date in a PNA homoduplex. The two bipyridines bulge out of the duplex and are aligned parallel to the major groove of the PNA. In addition, two bipyridines from adjacent PNA duplexes form a π-stacked pair that relates the duplexes within the crystal. The bulging out of the bipyridines causes bending of the PNA duplex, which is in contrast to the structure previously reported for biphenyl-modified DNA duplexes in solution, where the biphenyls are π stacked with adjacent nucleobase pairs and adopt an intrahelical geometry. This difference shows that relatively small perturbations can significantly impact the relative position of nucleobase analogues in nucleic acid duplexes.

摘要

肽核酸(PNA)是一种人工合成的 DNA 类似物,通常具有 N-氨乙基甘氨酸骨架。已经解决了两种 PNA 双链体的晶体结构,一种包含八个标准碱基对(GGCATGCC)(2),另一种包含相同的碱基对和中央对的联吡啶配体,分辨率分别为 1.22 和 1.10 Å。未修饰的 PNA 双链体采用类似于先前表征的 PNA 的 P 型螺旋结构。结构的原子级分辨率使我们能够首次观察到 PNA 末端赖氨酸与骨架和位于赖氨酸附近的碱基之间的特定相互作用模式,这被认为是诱导 PNA 双链体优选手性的重要因素。我们的结果支持这样的观点,即虽然 PNA 通常采用 P 型螺旋结构,但它的柔韧性相对较高。例如,含联吡啶的 PNA 的碱基对上升是迄今为止在 PNA 同源双链体中测量到的最大上升。两个联吡啶从双链体中突出,并与 PNA 的大沟平行排列。此外,相邻 PNA 双链体中的两个联吡啶形成π堆积对,将晶体中的双链体联系在一起。联吡啶的突出导致 PNA 双链体的弯曲,与先前在溶液中报告的联苯修饰的 DNA 双链体的结构形成对比,其中联苯与相邻的碱基对π堆积并采用腔内几何形状。这种差异表明,相对较小的干扰可以显著影响核酸双链体中碱基类似物的相对位置。

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