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Biomolecular Detection and Quantification最新文献

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How to make Mathematics Biology's next and better microscope 如何使数学生物学成为下一个更好的显微镜
Q1 Biochemistry, Genetics and Molecular Biology Pub Date : 2014-09-01 DOI: 10.1016/j.bdq.2014.09.001
Jim Huggett, Justin O’Grady, Stephen Bustin
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引用次数: 4
Determining lower limits of detection of digital PCR assays for cancer-related gene mutations 确定数字PCR检测癌症相关基因突变的下限
Q1 Biochemistry, Genetics and Molecular Biology Pub Date : 2014-09-01 DOI: 10.1016/j.bdq.2014.08.001
Coren A. Milbury , Qun Zhong , Jesse Lin, Miguel Williams, Jeff Olson, Darren R. Link, Brian Hutchison

Digital PCR offers very high sensitivity compared to many other technologies for processing molecular detection assays. Herein, a process is outlined for determining the lower limit of detection (LoD) of two droplet-based digital PCR assays for point mutations of the epidermal growth factor receptor (EGFR) gene. Hydrolysis probe mutation-detection assays for EGFR p.L858R and p.T790M mutations were characterized in detail. Furthermore, sixteen additional cancer-related mutation assays were explored by the same approach. For the EGFR L8585R assay, the assay sensitivity is extremely good, and thus, the LoD is limited by the amount of amplifiable DNA that is analyzed. With 95% confidence limits, the LoD is one mutant in 180,000 wild-type molecules for the evaluation of 3.3 μg of genomic DNA, and detection of one mutant molecule in over 4 million wild-type molecules was achieved when 70 million copies of DNA were processed. The measured false-positive rate for the EGFR L8585R assay is one in 14 million, which indicates the theoretical LoD if an unlimited amount of DNA is evaluated. For the EFGR T790M assay, the LoD is one mutant in 13,000 for analysis of a 3.3 μg sample of genomic DNA, and the dPCR assay limit sensitivity approaches one mutant in 22,000 wild-type molecules.

与许多其他处理分子检测分析的技术相比,数字PCR提供了非常高的灵敏度。本文概述了一种确定表皮生长因子受体(EGFR)基因点突变的两种基于液滴的数字PCR检测下限(LoD)的过程。水解探针突变检测方法对EGFR p.L858R和p.T790M突变进行了详细的表征。此外,采用相同的方法探索了另外16种与癌症相关的突变测定。对于EGFR L8585R检测,检测灵敏度非常好,因此,LoD受分析的可扩增DNA数量的限制。在95%置信限下,评估3.3 μg基因组DNA时,LoD为18万个野生型分子中1个突变体,处理7000万份DNA时,在400多万个野生型分子中检测到1个突变体。EGFR L8585R测定的假阳性率为1 / 1400万,这表明如果评估无限量的DNA,理论上的LoD。对于EFGR T790M分析,在3.3 μg基因组DNA样本中,LoD是13000个突变体中的一个,而dPCR分析的极限灵敏度接近22000个野生型分子中的一个突变体。
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引用次数: 146
Aims & Scope 目标及范围
Q1 Biochemistry, Genetics and Molecular Biology Pub Date : 2014-09-01 DOI: 10.1016/S2214-7535(14)00007-2
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引用次数: 0
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Biomolecular Detection and Quantification
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