在多种微小RNA(DQAMmiR)的直接定量分析中实现单核苷酸特异性
Achieving Single-Nucleotide Specificity in Direct Quantitative Analysis of Multiple MicroRNAs (DQAMmiR).
作者信息
Wegman David W, Ghasemi Farhad, Stasheuski Alexander S, Khorshidi Anna, Yang Burton B, Liu Stanley K, Yousef George M, Krylov Sergey N
机构信息
Department of Chemistry and Centre for Research on Biomolecular Interactions, York University , 4700 Keele Street, Toronto, Ontario M3J 1P3, Canada.
Sunnybrook Research Institute and Department of Laboratory Medicine and Pathobiology, Faculty of Medicine, University of Toronto , Toronto, Ontario M5S 1A8, Canada.
出版信息
Anal Chem. 2016 Feb 16;88(4):2472-7. doi: 10.1021/acs.analchem.5b04682. Epub 2016 Jan 26.
Direct quantitative analysis of multiple miRNAs (DQAMmiR) utilizes CE with fluorescence detection for fast, accurate, and sensitive quantitation of multiple miRNAs. Here we report on achieving single-nucleotide specificity and, thus, overcoming a principle obstacle on the way of DQAMmiR becoming a practical miRNA analysis tool. In general, sequence specificity is reached by raising the temperature to the level at which the probe-miRNA hybrids with mismatches melt while the matches remain intact. This elevated temperature is used as the hybridization temperature. Practical implementation of this apparently trivial approach in DQAMmiR has two major challenges. First, melting temperatures of all mismatched hybrids should be similar to each other and should not reach the melting temperature of any of the matched hybrids. Second, the elevated hybridization temperature should not deteriorate CE separation of the hybrids from the excess probes and the hybrids from each other. The second problem is further complicated by the reliance of separation in DQAMmiR on single-strand DNA binding protein (SSB) whose native structure and binding properties may be drastically affected by the elevated temperature. These problems were solved by two approaches. First, locked nucleic acid (LNA) bases were incorporated into the probes to normalize the melting temperatures of all target miRNA hybrids allowing for a single hybridization temperature; binding of SSB was not affected by LNA bases. Second, a dual-temperature CE was developed in which separation started with a high capillary temperature required for proper hybridization and continued at a low capillary temperature required for quality electrophoretic separation of the hybrids from excess probes and the hybrids from each other. The developed approach was sufficiently robust to allow its integration with sample preconcentration by isotachophoresis to achieve a limit of detection below 10 pM.
多种微小RNA的直接定量分析(DQAMmiR)利用带有荧光检测的毛细管电泳对多种微小RNA进行快速、准确且灵敏的定量分析。在此,我们报告实现了单核苷酸特异性,从而克服了DQAMmiR成为实用微小RNA分析工具道路上的一个主要障碍。一般来说,通过将温度升高到错配的探针 - 微小RNA杂交体解链而匹配的杂交体保持完整的水平来实现序列特异性。这个升高的温度用作杂交温度。在DQAMmiR中实际实施这种看似简单的方法有两个主要挑战。首先,所有错配杂交体的解链温度应彼此相似,且不应达到任何匹配杂交体的解链温度。其次,升高的杂交温度不应使杂交体与过量探针之间以及杂交体相互之间的毛细管电泳分离变差。DQAMmiR中的分离依赖于单链DNA结合蛋白(SSB),而升高的温度可能会极大地影响其天然结构和结合特性,这使得第二个问题更加复杂。通过两种方法解决了这些问题。首先,将锁核酸(LNA)碱基掺入探针中,以使所有靶标微小RNA杂交体的解链温度正常化,从而允许使用单一杂交温度;SSB的结合不受LNA碱基的影响。其次,开发了一种双温度毛细管电泳,其中分离开始于适当杂交所需的高毛细管温度,然后在将杂交体与过量探针以及杂交体相互之间进行高质量电泳分离所需的低毛细管温度下继续进行。所开发的方法足够稳健,能够与等速电泳样品预浓缩相结合,以实现低于10 pM的检测限。
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