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首页> 外文期刊>Clinical Chemistry: Journal of the American Association for Clinical Chemists >Probe-Free Digital PCR Quantitative Methodology to Measure Donor-Specific Cell-Free DNA after Solid-Organ Transplantation
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Probe-Free Digital PCR Quantitative Methodology to Measure Donor-Specific Cell-Free DNA after Solid-Organ Transplantation

机译:无探针数码PCR定量方法,以测量固体器官移植后测量供体的无细胞DNA

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BACKGROUND: Donor-specific cell-free DNA (dscfDNA) is increasingly being considered as a noninvasive biomarker to monitor graft health and diagnose graft rejection after solid-organ transplantation. However, current approaches used to measure dscfDNA can be costly and/or laborious. A probe-free droplet digital PCR (ddPCR) methodology using small deletion/insertion polymorphisms (DIPs) was developed to circumvent these limitations without compromising the quantification of dscfDNA. This method was called PHABRE-PCR (Primer to Hybridize across an Allelic BREakpoint-PCR). The strategic placement of one primer to hybridize across an allelic breakpoint ensured highly specific PCR amplification, which then enabled the absolute quantification of donor-specific alleles by probe-free ddPCR.
机译:背景:越来越多地被认为是富含供体的细胞DNA(DSCFDNA),以监测接枝健康和诊断接枝抑制固体器官移植后的非侵入性生物标志物。 然而,用于测量DSCFDNA的目前的方法可以是昂贵的和/或艰苦的。 使用小缺失/插入多态性(DIPS)的无探测液滴数码PCR(DDPCR)方法(DIPS)被开发,以避免这些限制而不损害DSCFDNA的定量。 该方法称为Phabre-PCR(引物以在等位基因断点-PCR上杂交)。 一种引物在等位基因断点中杂交的战略放置确保了高度特异性的PCR扩增,然后通过探针DDPCR使能量特异性等位基因的绝对量化。

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