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The replacement of cytogenetic analysis by direct chorionic villi sampling preparation with quantitative fluorescence PCR.

机译:用定量荧光PCR直接绒毛膜绒毛取样制备代替细胞遗传学分析。

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AIM: The aim of this study is to assess the replacement of chromosomal analysis of chorionic villi (CV) direct preparation samples (DIR) by quantitative fluorescence PCR (QF-PCR) and to determine its advantages in routine prenatal diagnosis. METHODS: From a total of 4,020 CV samples, rapid results were obtained either by conventional cytogenetic analysis of DIR in 2,770 samples, or by QF-PCR analysis in 1,250 samples. The final results were given after long-term culture (LTC). RESULTS: The frequencies of unbalanced fetal karyotypes were not significantly different, being 4.8% by DIR-LTC and 4.3% by QF-PCR-LTC. No false-negative or false-positive results were obtained from either approach. CONCLUSION: QF-PCR can replace chromosomal analysis of CV-DIR in most cases during routine prenatal diagnosis, requiring smaller CV samples and being more labor effective. Coupled with LTC, it is a robust diagnostic approach with high predictive value for the most frequent fetal trisomies.
机译:目的:本研究旨在评估通过定量荧光PCR(QF-PCR)替代绒毛膜(CV)直接制备样品(DIR)的染色体分析,并确定其在常规产前诊断中的优势。方法:从总共4,020个CV样本中,通过常规的2770个样本的DIR的细胞遗传学分析或通过1,250个样本的QF-PCR分析获得了快速的结果。长期培养(LTC)后得出最终结果。结果:胎儿核型不平衡的频率无明显差异,DIR-LTC为4.8%,QF-PCR-LTC为4.3%。两种方法均未获得假阴性或假阳性结果。结论:在常规产前诊断中,大多数情况下,QF-PCR可以代替CV-DIR的染色体分析,所需的CV样本更少,劳动效率更高。与LTC结合使用,它是一种可靠的诊断方法,对最常见的胎儿三体性疾病具有较高的预测价值。

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