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Modified peptide nucleic acids (PNA) and amonafide derivatives: Synthesis and applications of trans-cyclopentane and trans-pyrrolidine PNAs and small molecules derived from amonafide.

机译:修饰的肽核酸(PNA)和阿莫那肽衍生物:反式环戊烷和反吡咯烷PNA以及阿莫那肽衍生的小分子的合成和应用。

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摘要

Peptide nucleic acids were discovered by Nielsen and coworkers in 1991 as nucleic acid analogues where the sugar-phosphate backbone is replaced with an uncharged, achiral backbone. PNAs hybridize to complementary DNA and RNA via Watson-Crick hydrogen bonds with higher affinity than corresponding oligonucleotides. These properties make PNA a promising molecule for DNA diagnostic and biological applications. In unmodified PNAs, the aminoethyl-glycine backbone is flexible and, as a result, there is entropic loss associated with duplex formation. The incorporation of (S,S)-trans-1,2-cyclopentane diamine into the PNA backbone increases the binding affinity compared to unmodified PNAs, due to a decrease in entropic loss. Efficient synthetic routes to cyclopentane PNA monomers containing the four standard DNA nucleobases have been developed. These monomers have then been incorporated into PNA strands utilizing a mixed protecting group strategy, and have shown increases in binding affinity and sequence specifity in comparison to unmodified PNA strands. Similar to the (S,S)-trans-1,2-cyclopentane PNA, ( S,S)-trans-pyrrolidine modified PNAs showed an increase in binding affinity and sequence specificty. The (S,S)- trans-pyrrolidine PNA should aid in aqueous solubility, an aspect of PNA technology that can be problematic.; To prepare PNA monomers containing guanine, it was necessary to prepare N-9 guanine acetic acid. Methodology to produce either the N-9 or N-7 alkylated guanine has been developed. The N-7 alkylated product can be incorporated into PNA monomers and used as a protonated cytosine mimic. Insertion of N-7 alkylated guanine monomers into the Hoogsteen binding strand of bis-PNA hairpins produces compounds that can undergo strand invasion of double stranded DNA, forming a stable PNA2/DNA triplex. By installing a fluorescent probe onto the bis-PNA hairpin, it is possible to mark plasmid DNA and monitor its migration through the cell.; An efficient 2-step synthetic route to 4-substituted amonafide derivatives was developed. The synthesis allowed for a wide range of analogues to be prepared quickly and also allowed for the cursory production of multi-gram quantities of amonafide analogues. These molecules were tested for anticancer activity in collaboration with Professor Sui Huang at Northwestern Medical School.
机译:肽核酸是Nielsen及其同事在1991年发现的核酸类似物,其中糖-磷酸骨架被不带电荷的非手性骨架取代。 PNA通过Watson-Crick氢键与互补的DNA和RNA杂交,其亲和力高于相应的寡核苷酸。这些特性使PNA成为用于DNA诊断和生物学应用的有前途的分子。在未修饰的PNA中,氨乙基-甘氨酸主链是柔性的,因此,存在与双链体形成相关的熵损失。由于熵损失的减少,与未修饰的PNA相比,将(S,S)-反-1,2-环戊烷二胺掺入PNA主链可增加结合亲和力。已经开发出有效的合成路线,以合成含有四个标准DNA核碱基的环戊烷PNA单体。然后利用混合保护基策略将这些单体掺入PNA链中,与未修饰的PNA链相比,它们的结合亲和力和序列特异性提高。与(S,S)-反式-1,2-环戊烷PNA相似,(S,S)-反式吡咯烷修饰的PNA显示结合亲和力和序列特异性增加。 (S,S)-反吡咯烷PNA应有助于水溶性,这是PNA技术的一个方面。为了制备含有鸟嘌呤的PNA单体,必须制备N-9鸟嘌呤乙酸。已经开发出生产N-9或N-7烷基化鸟嘌呤的方法。 N-7烷基化产物可以掺入PNA单体中,并用作质子化胞嘧啶模拟物。将N-7烷基化的鸟嘌呤单体插入bis-PNA发夹的Hoogsteen结合链中会产生可经历双链DNA链入侵的化合物,形成稳定的PNA2 / DNA三链体。通过将荧光探针安装在bis-PNA发夹上,可以标记质粒DNA并监测其在细胞中的迁移。开发了一种有效的2步合成4取代amonafide衍生物的途径。该合成使得可以快速制备多种类似物,并且还可以粗略生产数克量的阿莫奈德类似物。与西北医学院的黄穗教授合作测试了这些分子的抗癌活性。

著录项

  • 作者

    Witschi, Mark Andre.;

  • 作者单位

    Northwestern University.;

  • 授予单位 Northwestern University.;
  • 学科 Chemistry Organic.
  • 学位 Ph.D.
  • 年度 2006
  • 页码 154 p.
  • 总页数 154
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 有机化学;
  • 关键词

  • 入库时间 2022-08-17 11:40:20

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