首页> 外文期刊>Talanta: The International Journal of Pure and Applied Analytical Chemistry >Ultra-fast separation of infectious disease-related small DNA molecules by single- and multi-channel microchip electrophoresis
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Ultra-fast separation of infectious disease-related small DNA molecules by single- and multi-channel microchip electrophoresis

机译:通过单通道和多通道微芯片电泳超快分离与传染病相关的小DNA分子

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摘要

An ultra-fast and precise microchip electrophoresis (ME) method was developed for the separation of infectious disease-related small DNA molecules. As a model of infectious disease-related small DNA molecules, the spike glycoprotein (S) gene of the Feline infectious peritonitis (FIP) virus was amplified using reverse transcript polymerase chain reaction. The amplified product of the FIP virus (223-bp) was analyzed within 10 s by single-channel ME under a sieving gel of 0.3% poly(ethylene oxide) (M_r=8,000,000) in lx TBE buffer (pH 8.33) and a short effective channel length of 1.3 cm with a programmed step electric field strength (PSEFS) condition as follows: 470.6 V/cm for 9 s, 294.1 V/cm 1.5 s, and 470.6 V/cm for 9.5 s. The single-channel ME/PSEFS method was 50 times faster than that obtained with conventional slab gel electrophoresis. When the single-channel ME method was applied to a multi-channel ME for high-throughput screening, the precision of migration time and peak area showed standard deviations of less than 1.0% without any loss of resolving power. The ME assay technique provides a simple, precise and accurate method for ultra-fast analysis of infectious disease-related DNA under 400-bp.
机译:开发了一种用于分离与传染病相关的小DNA分子的超快速,精确的微芯片电泳(ME)方法。作为与传染病相关的小DNA分子的模型,猫传染性腹膜炎(FIP)病毒的棘突糖蛋白(S)基因通过逆转录聚合酶链反应扩增。在1x TBE缓冲液(pH 8.33)中,在0.3%聚环氧乙烷(M_r = 8,000,000)的筛分凝胶下,通过单通道ME在10 s内分析了FIP病毒的扩增产物(223-bp)。编程的步进电场强度(PSEFS)条件如下所示,有效通道长度为1.3 cm:470.6 V / cm持续9 s,294.1 V / cm 1.5 s和470.6 V / cm持续9.5 s。单通道ME / PSEFS方法比常规平板凝胶电泳方法快50倍。当单通道ME方法应用于多通道ME进行高通量筛选时,迁移时间和峰面积的精度显示标准偏差小于1.0%,而没有任何分离度损失。 ME分析技术为400 bp以下的传染病相关DNA的超快速分析提供了一种简单,精确和准确的方法。

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