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嵌合 γPNA-Invader 探针:利用嵌入剂功能化寡核苷酸增强 γPNA 的 DNA 靶向特性。

Chimeric γPNA-Invader probes: using intercalator-functionalized oligonucleotides to enhance the DNA-targeting properties of γPNA.

机构信息

Department of Chemistry, University of Idaho, Moscow, ID-83844, USA.

出版信息

Org Biomol Chem. 2020 Feb 21;18(7):1359-1368. doi: 10.1039/c9ob02726b. Epub 2020 Jan 27.

DOI:10.1039/c9ob02726b
PMID:31984413
Abstract

Gamma peptide nucleic acids (γPNAs), i.e., single-stranded PNA strands that are modified at the γ-position with (R)-diethylene glycol, and Invader probes, i.e., DNA duplexes with +1 interstrand zipper arrangements of 2'-O-(pyren-1-yl)methyl-RNA monomers, are two types of nucleic acid mimics that are showing promise for sequence-unrestricted recognition of double-stranded (ds) DNA targets. We recently demonstrated that recognition of dsDNA targets with self-complementary regions is challenging for single-stranded high-affinity probes like γPNAs due to their proclivity for secondary structure formation, but not so for Invader probes, which are engineered to form readily denaturing duplexes irrespective of the target sequence context. In the present study, we describe an approach that mitigates these limitations and improves the dsDNA-recognition properties of γPNAs in partially self-complementary target contexts. Chimeric probes between γPNAs and individual Invader strands are shown to form metastable duplexes that (i) are energetically activated for recognition of complementary mixed-sequence dsDNA target regions, (ii) reduce γPNA dimerization, and (iii) substantially improve the fidelity of the dsDNA-recognition process. Chimeric γPNA-Invader probes are characterized with respect to thermal denaturation properties, thermodynamic parameters associated with duplex formation, UV-Vis and fluorescence trends to establish pyrene binding modes, and dsDNA-recognition properties using DNA hairpin model targets.

摘要

伽马肽核酸(γPNAs),即 γ 位经(R)-二甘醇修饰的单链 PNA 链,和侵入探针,即具有+1 链间拉链排列的 2'-O-(吡嗪-1-基)甲基-RNA 单体的 DNA 双链体,是两种核酸类似物,它们在序列不受限制的识别双链 (ds) DNA 靶标方面显示出了前景。我们最近证明,对于自我互补区域的 dsDNA 靶标,具有自我互补区域的 dsDNA 靶标的识别对于单链高亲和力探针(如 γPNAs)具有挑战性,这是由于它们倾向于形成二级结构,但对于 Invader 探针则不然,Invader 探针被设计为形成易于变性的双链体,而不管靶序列上下文如何。在本研究中,我们描述了一种方法,该方法可以减轻这些限制并改善部分自我互补靶标环境中 γPNAs 的 dsDNA 识别特性。γPNAs 和单个侵入探针之间的嵌合探针被证明可以形成亚稳态双链体,这些双链体 (i) 可被能量激活以识别互补的混合序列 dsDNA 靶区,(ii) 减少 γPNA 二聚化,和 (iii) 极大地提高 dsDNA 识别过程的保真度。用 DNA 发夹模型靶标,对嵌合 γPNA-Invader 探针进行了热变性特性、双链体形成相关热力学参数、UV-Vis 和荧光趋势以建立吡嗪结合模式以及 dsDNA 识别特性的表征。

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