Droplet digital PCR improves urinary exosomal miRNA detection compared to real-time PCR.

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2019

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Abstract

Quantification of urinary miRNAs can be challenging especially for low abundance miRNAs. We aimed to optimize the quantification of urinary exosomal miRNAs and compare the performance efficiency between droplet digital PCR (ddPCR) and real-time quantitative PCR (qPCR).We optimized a number of parameters for ddPCR such as annealing temperatures, annealing time and PCR cycle number. We also compared the performance of ddPCR and qPCR.By comparing the fluorescence amplification separation, the optimal annealing temperature was 59 °C, optimal annealing time was 60s and optimal cycle number was 45 for measuring urinary exosomal miRNAs. ddPCR had much higher technical sensitivity compared to qPCR. The minimal detectable concentration of miR-29a was <50 copies/μL by ddPCR compared to 6473 copies/μL for qPCR. Also, ddPCR generated more consistent results for serially diluted samples compared to qPCR. ddPCR generated smaller within-run variations than qPCR though this did not reach statistical significance. It also resulted in better reproducibility with smaller between-run variations.Optimization of urinary exosomal miRNA ddPCR assay is dependent on assessing key variables including experimental annealing temperature and time as well as the number of PCR cycles. ddPCR has a higher sensitivity, reproducibility, and accuracy in comparison to qPCR.

Reference Key	wang2019dropletclinical Use this key to autocite in the manuscript while using SciMatic Manuscript Manager or Thesis Manager
Authors	Wang, Cong;Ding, Qiang;Plant, Pamela;Basheer, Mayada;Yang, Chuance;Tawedrous, Eriny;Krizova, Adriana;Boulos, Carl;Farag, Mina;Cheng, Yufeng;Yousef, George M;
Journal	Clinical biochemistry
Year	2019
DOI	S0009-9120(18)30907-X
URL	https://doi.org/S0009-9120(18)30907-X
Keywords	optimization exosome qpcr mirna urine ddpcr abbreviations droplet digital polymerase chain reaction quantitative real time polymerase chain reaction

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