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首页> 外文期刊>Annals of the New York Academy of Sciences >Optimized Real-Time Quantitative PCR Measurement of Male Fetal DNA in Maternal Plasma
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Optimized Real-Time Quantitative PCR Measurement of Male Fetal DNA in Maternal Plasma

机译:母体血浆中男性胎儿DNA的实时荧光定量PCR优化检测

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摘要

DNA of fetal origin is present in the plasma of pregnant women. The quantitative measurement of circulatory fetal DNA (cfDNA) by real-time quantitative PCR (qPCR) has been applied to investigate a possible correlation between increased levels and pregnancy-related disorders. However, as the levels of cfDNA are close to the detection limit (LOD) of the method used, the measurements may not be reliable. This is also problematic for the evaluation of preanalytical steps, such as DNA extraction and cfDNA enrichment by size separation. We optimized a protocol for the qPCR analysis of the multi-copy sequence DYS14 on the Y chromosome. This was compared with an established assay for the single-copy SRY gene. Probit regression analysis showed that the limit of detection (LOD) of the DYS14 assay, (0.4 genome equivalents (GE)) and limit of quantification (LOQ) were 10-fold lower in comparison to SRY (4 GE). The levels of cfDNA obtained from the first trimester of pregnancy could be quantified with high precision by the DYS14 assay (CV below 25%) as opposed to the SRY measurements (26-140%). Additionally, fetal sex was correctly determined in all instances. The low copy numbers of fetal DNA in plasma of women in the first trimester of pregnancy can be measured reliably, targeting the DYS14 that is present in multiple copies per Y chromosome.
机译:胎儿血浆中存在胎儿来源的DNA。通过实时定量PCR(qPCR)对循环胎儿DNA(cfDNA)的定量测​​量已用于研究血脂水平升高与妊娠相关疾病之间的可能相关性。但是,由于cfDNA的水平接近所用方法的检测极限(LOD),因此测量可能不可靠。这对于分析前步骤的评估也是有问题的,例如通过大小分离进行DNA提取和cfDNA富集。我们优化了用于Y染色体上的多拷贝序列DYS14的qPCR分析的协议。将其与单拷贝SRY基因的既定测定法进行比较。概率回归分析表明,与SRY(4 GE)相比,DYS14分析的检测极限(LOD)(0.4基因组当量(GE))和定量极限(LOQ)低10倍。可以通过DYS14测定(CV低于25%)和SRY测量(26-140%)以高精度对从妊娠头三个月获得的cfDNA进行定量。此外,在所有情况下都正确确定了胎儿性别。可以可靠地检测出孕妇妊娠早期血浆中胎儿DNA的低拷贝数,靶向每个Y染色体中存在多个拷贝的DYS14。

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