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Evaluation of Digital PCR for Absolute DNA Quantification

机译:评估数字PCR绝对DNA定量

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The emerging technique of microfluidic digital PCR (dPCR) offers a unique approach to real-time quantitative PCR for measuring nucleic acids that may be particularly suited for low-level detection. In this study, we evaluated the quantitative capabilities of dPCR when measuring small amounts (<200 copies) of DNA and investigated parameters influencing technical performance. We used various DNA templates, matrixes, and assays to evaluate the precision, sensitivity and reproducibility of dPCR, and demonstrate that this technique can be highly reproducible when performed at different times and when different primer sets are targeting the same molecule. dPCR exhibited good analytical sensitivity and was reproducible outside the range recommended by the instrument manufacturer; detecting 16 estimated targets with high precision. The inclusion of carrier had no effect on this estimated quantity, but did improve measurement precision. We report disagreement when using dPCR to measure different template types and when comparing the estimated quantities by dPCR and UV spectrophotometry. Finally, we also demonstrate that preamplification can impose a significant measurement bias. These findings provide an independent assessment of low copy molecular measurement using dPCR and underline important factors for consideration in dPCR experimental design.
机译:新兴的微流数字PCR(dPCR)技术为实时定量PCR提供了一种独特的方法来测量可能特别适合于低水平检测的核酸。在这项研究中,我们评估了当测量少量(<200拷贝)DNA时dPCR的定量能力,并研究了影响技术性能的参数。我们使用了各种DNA模板,基质和测定法来评估dPCR的准确性,敏感性和可重复性,并证明了该技术在不同时间执行且不同引物组针对同一分子时可以高度重现。 dPCR表现出良好的分析灵敏度,并且可在仪器制造商建议的范围之外重现;高精度检测16个估计目标。包含载体对此估计量没有影响,但确实提高了测量精度。当使用dPCR测量不同模板类型以及通过dPCR和紫外分光光度法比较估计数量时,我们报告了分歧。最后,我们还证明了前置放大可以施加明显的测量偏差。这些发现为使用dPCR的低拷贝分子测量提供了独立评估,并强调了在dPCR实验设计中需要考虑的重要因素。

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