首页> 美国卫生研究院文献>BioMed Research International >Whole Genome Amplification of Day 3 or Day 5 Human Embryos Biopsies Provides a Suitable DNA Template for PCR-Based Techniques for Genotyping, a Complement of Preimplantation Genetic Testing
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Whole Genome Amplification of Day 3 or Day 5 Human Embryos Biopsies Provides a Suitable DNA Template for PCR-Based Techniques for Genotyping, a Complement of Preimplantation Genetic Testing

机译:第3天或第5天人类胚胎活检的全基因组扩增为基于PCR的基因分型技术提供了合适的DNA模板,这是对植入前基因测试的补充

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摘要

Our objective was to determine if whole genome amplification (WGA) provides suitable DNA for qPCR-based genotyping for human embryos. Single blastomeres (Day 3) or trophoblastic cells (Day 5) were isolated from 342 embryos for WGA. Comparative Genomic Hybridization determined embryo sex as well as Trisomy 18 or Trisomy 21. To determine the embryo's sex, qPCR melting curve analysis for SRY and DYS14 was used. Logistic regression indicated a 4.4%, 57.1%, or 98.8% probability of a male embryo when neither gene, SRY only, or both genes were detected, respectively (accuracy = 94.1%, kappa = 0.882, and p < 0.001). Fluorescent Capillary Electrophoresis for the amelogenin genes (AMEL) was also used to determine sex. AMELY peak's height was higher and this peak's presence was highly predictive of male embryos (AUC = 0.93, accuracy = 81.7%, kappa = 0.974, and p < 0.001). Trisomy 18 and Trisomy 21 were determined using the threshold cycle difference for RPL17 and TTC3, respectively, which were significantly lower in the corresponding embryos. The Ct difference for TTC3 specifically determined Trisomy 21 (AUC = 0.89) and RPL17 for Trisomy 18 (AUC = 0.94). Here, WGA provides adequate DNA for PCR-based techniques for preimplantation genotyping.
机译:我们的目标是确定全基因组扩增(WGA)是否为​​人类胚胎基于qPCR的基因分型提供合适的DNA。从WGA的342个胚胎中分离出单个卵裂球(第3天)或滋养细胞(第5天)。比较基因组杂交确定了胚胎的性别以及18三体或21三体。为了确定胚胎的性别,使用了SRY和DYS14的qPCR熔解曲线分析。 Logistic回归表明,分别未检测到基因,仅SRY或同时检测到两个基因时,男性胚胎的概率分别为4.4%,57.1%或98.8%(准确性= 94.1%,κ= 0.882和p <0.001)。釉蛋白原基因(AMEL)的荧光毛细管电泳也用于确定性别。 AMELY峰的高度更高,并且该峰的存在可高度预测雄性胚胎(AUC = 0.93,准确度= 81.7%,kappa = 0.974,p <0.001)。分别使用RPL17和TTC3的阈值循环差异确定18三体性和21三体性,这在相应的胚胎中明显较低。 TTC3的Ct差异具体确定了21三体(AUC = 0.89),RPL17的三体18(AUC = 0.94)。在这里,WGA为基于PCR的技术进行植入前基因分型提供了足够的DNA。

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