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Peptide nucleic acids (PNA) derived from N-(N-methylaminoethyl)glycine. Synthesis, hybridization and structural properties

机译:衍生自N-(N-甲基氨基乙基)甘氨酸的肽核酸(PNA)。合成,杂交和结构性质

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摘要

Backbone N-methylated peptide nucleic acids (PNAs) containing the four nucleobases adenine, cytosine, guanine and thymine were synthesized via solid phase peptide oligomerization. The oligomers bind to their complementary target with a thermal stability that is 1.5–4.5°C lower per "N-methyl nucleobase unit' [dependent on the number and position(s) of the N-methyl] than that of unmodified PNA. However, even fully N-methyl modified PNAs bind as efficiently to DNA or RNA targets as DNA itself. Furthermore, the hybridization efficiency per N-methyl unit in a PNA decreased with increasing N-methyl content, and the effect was more pronounced when the N-methyl backbone units are present in the Hoogsteen versus the Watson–Crick strand in (PNA)2-DNA triplexes. Interestingly, CD spectral analyses indicate that 30% (3 out of ten) substitution with N-methyl nucleobases did not alter the structure of PNA-DNA (or RNA) duplexes or (PNA)2-DNA triplexes, and likewise CD spectroscopy and X-ray crystallography showed no major structural differences between N-methylated (30%) and unmodified PNA-PNA duplexes. However, PNA-DNA duplexes as well as triplexes adopted a different conformation when formed with all-N-methyl PNAs.
机译:通过固相肽寡聚合成包含四个核碱基腺嘌呤,胞嘧啶,鸟嘌呤和胸腺嘧啶的骨干N-甲基化肽核酸(PNA)。低聚物以其“ N-甲基核碱基单位”(取决于N-甲基的数目和位置)低1.5-4.5°C的热稳定性结合其互补靶标,这一点比未修饰的PNA要低。 ,甚至完全被N-甲基修饰的PNA与DNA或DNA靶一样有效地结合到DNA或RNA靶上,而且,随着N-甲基含量的增加,PNA中每个N-甲基单元的杂交效率降低,当N -甲基骨架单元位于(PNA)2-DNA三元组的Hoogsteen与Watson-Crick链中,有趣的是,CD光谱分析表明,N-甲基核碱基取代了30%(十分之三)不会改变结构PNA-DNA(或RNA)双链体或(PNA)2-DNA三链体的分离,CD光谱法和X射线晶体学分析也显示N-甲基化(30%)和未修饰的PNA-PNA双链体之间无主要结构差异。 -DNA双链体和三链体采用不同的构型与全N-甲基PNA结合时的反应

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