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首页> 外文期刊>Nucleic Acids Research >Microchip electrophoresis: a method for high-speed SNP detection.
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Microchip electrophoresis: a method for high-speed SNP detection.

机译:微芯片电泳:一种用于高速SNP检测的方法。

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摘要

As a trial practical application, we have applied optimized microfabricated electrophoresis devices, combined with enzymatic mutation detection methods, to the determination of single nucleotide polymorphism (SNP) sites in the p53 suppressor gene. Using clinical samples, we have achieved robust assays with quality factors as good as conventional electrophoresis in approximately 100 s. This is 10 and 50 times faster than capillary and slab gel electro-phoresis, respectively. The method was highly accurate with an average error of mutation site measurement of only +/-5 bp. No clean-up of the digestion mixtures was needed prior to injection. This greatly simplifies sample handling relative to capillary instruments, which is important for high-throughput screening applications. Following identification, absolute mutation determination of the screened samples was achieved in a second microdevice optimized for four-color DNA sequencing. Total run time was 25 min in this second device and sequencing data were in full agreement with ABI Prism 377 sequencing runs which required 3.5 h. The tandem application of microdevices for location then full characterization of SNPs appears to confirm many of the improvements claimed for future application of microdevices in practical scaled screening for mutational analysis.
机译:作为试验性的实际应用,我们将优化的微细电泳设备与酶促突变检测方法结合使用,以确定p53抑制基因中的单核苷酸多态性(SNP)位点。使用临床样品,我们在大约100 s内就获得了质量因子与常规电泳一样好的鲁棒测定。这分别比毛细管电泳和平板凝胶电泳快10到50倍。该方法非常准确,突变位点测量的平均误差仅为+/- 5 bp。注射前无需清除消化混合物。相对于毛细管仪器,这大大简化了样品处理,这对于高通量筛选应用非常重要。鉴定后,在优化用于四色DNA测序的第二个微型设备中实现了筛选样品的绝对突变测定。第二台设备的总运行时间为25分钟,测序数据与ABI Prism 377测序运行完全一致,需要3.5小时。串联使用微型设备进行定位,然后对SNPs进行全面表征,似乎证实了对微型设备在突变分析的实际规模筛选中未来应用的许多改进。

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