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Amplified Single Base-Pair Mismatch Detection via Aggregation of Exonuclease-Sheared Gold Nanoparticles

机译:通过核酸外切酶剪切的金纳米粒子的聚集的单碱基对错配扩增检测。

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摘要

Single nucleotide polymorphism (SNP) detection is important for early diagnosis, clinical prognostics, and disease prevention, and a rapid and sensitive low-cost SNP detection assay would be valuable for resource-limited clinical settings. We present a simple platform that enables sensitive, naked-eye detection of SNPs with minimal reagent and equipment requirements at room temperature within 15 min. SNP detection is performed in a single tube with one set of DNA probe-modified gold nanoparticles (AuNPs), a single exonuclease (Exo III), and the target in question. Exo III's apurinic endonucleolytic activity differentially processes hybrid duplexes between the AuNP-bound probe and DNA targets that are perfectly matched or contain a single-base mismatch. For perfectly matched targets, Exo III's exonuclease activity facilitates a process of target recycling that rapidly shears DNA probes from the particles, generating an AuNP aggregation-induced color change, whereas no such change occurs for mismatched targets. This color change is easily observed with as little as 2 nM of target, 100-fold lower than the target concentration required for reliable naked eye observation with unmodified AuNPs in well-optimized reaction conditions. We further demonstrate that this system can effectively discriminate a range of different mismatches.
机译:单核苷酸多态性(SNP)检测对于早期诊断,临床预后和疾病预防非常重要,而快速且灵敏的低成本SNP检测测定对于资源有限的临床环境将非常有价值。我们提供了一个简单的平台,可以在室温下15分钟内用最少的试剂和设备要求,以肉眼检测SNP。 SNP检测是在带有一组DNA探针修饰的金纳米颗粒(AuNPs),单个核酸外切酶(Exo III)和相关靶标的单管中进行的。 Exo III的嘌呤内切核酸酶活性不同地处理了AuNP结合的探针和完全匹配或包含单碱基错配的DNA靶之间的杂交双链体。对于完全匹配的靶标,Exo III的核酸外切酶活性促进了靶标回收的过程,该过程可从颗粒中快速剪切DNA探针,产生AuNP聚集诱导的颜色变化,而错配的靶标则不会发生这种变化。仅需2 nM的目标分子即可轻松观察到这种颜色变化,这比在优化的反应条件下使用未修饰的AuNP进行可靠的肉眼观察所需的目标浓度低100倍。我们进一步证明,该系统可以有效地区分一系列不同的不匹配项。

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