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Determination of fetal aneuploidies by massively parallel DNA sequencing

机译:大规模平行DNA测序测定胎儿非整倍性

摘要

The present methods are exemplified by a process in which maternal blood containing fetal DNA is diluted to a nominal value of approximately 0.5 genome equivalent of DNA per reaction sample. Digital PCR is then be used to detect aneuploidy, such as the trisomy that causes Down Syndrome. Since aneuploidies do not present a mutational change in sequence, and are merely a change in the number of chromosomes, it has not been possible to detect them in a fetus without resorting to invasive techniques such as amniocentesis or chorionic villi sampling. Digital amplification allows the detection of aneuploidy using massively parallel amplification and detection methods, examining, e.g., 10,000 genome equivalents.
机译:本方法通过以下方法举例说明,其中将含有胎儿DNA的母体血液稀释至每个反应样品的DNA的基因组当量约0.5的标称值。然后使用数字PCR检测非整倍性,例如引起唐氏综合症的三体性。由于非整倍体不会在序列上呈现突变变化,而仅仅是染色体数目的变化,因此如果不借助羊膜穿刺术或绒毛膜绒毛取样等侵入性技术,就不可能在胎儿中检测到它们。数字扩增允许使用大规模平行扩增和检测方法检测非整倍性,例如检查10,000个基因组当量。

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