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首页> 外文期刊>Biomacromolecules >High Affinity γPNA Sandwich Hybridization Assay for Rapid Detection of Short Nucleic Acid Targets with Single Mismatch Discrimination
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High Affinity γPNA Sandwich Hybridization Assay for Rapid Detection of Short Nucleic Acid Targets with Single Mismatch Discrimination

机译:高亲和力γPNA夹心杂交技术可快速检测具有单个错配识别的短核酸靶标

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摘要

Hybridization analysis of short DNA and RNA targets presents many challenges for detection. The commonly employed sandwich hybridization approach cannot be implemented for these short targets due to insufficient probe-target binding strengths for umnodified DNA probes. Here, we present a method capable of rapid and stable sandwich hybridization detection for 22 nucleotide DNA and RNA targets. Stable hybridization is achieved using an n-alkylated, polyethylene glycol γ-carbon modified peptide nucleic acid (γPNA) amphiphile. The γPNA's exceptionally high affinity enables stable hybridization of a second DNA-based probe to the remaining bases of the short target. Upon hybridization of both probes, an electrophoretic mobility shift is measured via interaction of the n-alkane modification on the γPNA with capillary electrophoresis running bufier containing nonionic surfactant micelles. We find that sandwich hybridization of both probes is stable under multiple binding configurations and demonstrate single base mismatch discrimination. The binding strength of both probes is also stabilized via coaxial stacking on adjacent hybridization to targets. We conclude with a discussion on the implementation of the proposed sandwich hybridization assay as a high-throughput microRNA detection method.
机译:短DNA和RNA靶标的杂交分析对检测提出了许多挑战。由于这些未标记的DNA探针的探针-靶标结合强度不足,因此无法对这些短靶标实施常用的夹心杂交方法。在这里,我们提出了一种能够对22个核苷酸的DNA和RNA靶标进行快速,稳定的三明治杂交检测的方法。使用正烷基化的聚乙二醇γ-碳修饰的肽核酸(γPNA)两亲物可实现稳定的杂交。 γPNA的超高亲和力使第二个基于DNA的探针与短靶标的其余碱基稳定杂交。两种探针均杂交后,通过在γPNA上进行正构烷烃修饰与毛细管电泳(包含非离子表面活性剂胶束的毛细管电泳)相互作用来测量电泳迁移率变化。我们发现两种探针的三明治杂交在多种结合构型下都是稳定的,并证明了单碱基错配的鉴别。通过与靶标相邻杂交时的同轴堆叠,两种探针的结合强度也得以稳定。最后,我们讨论了拟议的夹心杂交测定法作为高通量microRNA检测方法的实施。

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