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金纳米颗粒上核酸的酶促切割:用于简便比色生物传感器的通用平台。

Enzymatic cleavage of nucleic acids on gold nanoparticles: a generic platform for facile colorimetric biosensors.

作者信息

Zhao Weian, Lam Jeffrey C F, Chiuman William, Brook Michael A, Li Yingfu

机构信息

Department of Chemistry, McMaster University, 1280 Main St. West, Hamilton, ON L8S 4M1, Canada.

出版信息

Small. 2008 Jun;4(6):810-6. doi: 10.1002/smll.200700757.

Abstract

The enzymatic cleavage of nucleic acids (DNA or DNA with a single RNA linkage) on well-dispersed gold nanoparticles (AuNPs) is exploited in the design of facile colorimetric biosensors. The assays are performed at salt concentrations such that DNA-modified AuNPs are barely stabilized by the electrostatic and steric stabilization. Enzymatic cleavage of DNA chains on the AuNP surface destabilizes the AuNPs, resulting in a rapid aggregation driven by van der Waals attraction, and a red-to-purple color change. Two different systems are chosen, DNase I (a DNA endonuclease) and 8-17 (a Pb(2+)-depedent RNA-cleaving DNAzyme), to demonstrate the utility of our assay for the detection of metal ions and sensing enzyme activities. Compared with previous studies in which AuNP aggregates are converted into dispersed AuNPs by enzymatic cleavage of DNA crosslinkers, the present assay is technically simpler. Moreover, the accessibility of DNA to biomolecular recognition elements (e.g. enzymes) on well-dispersed AuNPs in our assay appears to be higher than that embedded inside aggregates. This biosensing system should be readily adaptable to other enzymes or substrates for detection of analytes such as small molecules, proteases and their inhibitors.

摘要

在设计简便的比色生物传感器时,利用了核酸(DNA或带有单个RNA连接的DNA)在高度分散的金纳米颗粒(AuNP)上的酶促切割。这些测定是在盐浓度下进行的,使得DNA修饰的AuNP几乎不能通过静电和空间稳定作用而稳定。AuNP表面上DNA链的酶促切割使AuNP不稳定,导致由范德华引力驱动的快速聚集,并发生从红色到紫色的颜色变化。选择了两种不同的系统,即DNase I(一种DNA内切酶)和8-17(一种依赖Pb(2+)的RNA切割DNA酶),以证明我们的测定法在检测金属离子和传感酶活性方面的实用性。与先前将DNA交联剂酶促切割使AuNP聚集体转化为分散的AuNP的研究相比,本测定法在技术上更简单。此外,在我们的测定法中,DNA对高度分散的AuNP上的生物分子识别元件(例如酶)的可及性似乎高于嵌入聚集体内部的DNA。这种生物传感系统应该很容易适用于其他酶或底物,以检测诸如小分子、蛋白酶及其抑制剂等分析物。

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