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Rapid Prenatal Diagnosis by QF-PCR: Evaluation of 30,000 Consecutive Clinical Samples and Future Applications

机译:通过QF-PCR快速进行产前诊断:30,000份连续临床样品的评估和未来应用

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摘要

Rapid prenatal diagnoses of major chromosome abnormalities can be performed on a large scale using highly polymorphic short tandem repeats (STRs) amplified by the quantitative fluorescent polymerase chain reaction (QF-PCR). The assay was introduced as a preliminary investigation to remove the anxiety of the parents waiting for the results by conventional cytogenetic analysis using amniotic fluid or chorionic cells. However, recent studies, on the basis of the analyses of several thousand samples, have shown that this rapid approach has a very high rate of success and could reduce the need for cytogenetic investigations. Its high efficiency, for example, allows early interruption of affected fetuses without the need of waiting for completion of fetal karyotype. The main advantages of the QF-PCR are its accuracy, speed, automation, and low cost that allows very large number of samples to be analyzed by few operators. Here, we report the results of using QF-PCR in a large series of consecutive clinical cases and discuss the possibility that, in a near future, it may even replace conventional cytogenetic analyses on selected samples.
机译:可以使用通过定量荧光聚合酶链反应(QF-PCR)扩增的高度多态性的短串联重复序列(STR),大规模进行快速的产前诊断,以进行主要染色体异常的诊断。该测定法是一种初步研究,旨在通过使用羊水或绒毛膜细胞的常规细胞遗传学分析消除等待结果的父母的焦虑。但是,根据对数千个样品的分析,最近的研究表明,这种快速方法具有很高的成功率,并且可以减少细胞遗传学研究的需要。例如,它的高效率可以使受影响的胎儿早日中断,而无需等待胎儿核型的完成。 QF-PCR的主要优势在于它的准确性,速度,自动化和低成本,这使得极少的操作员能够分析大量样品。在这里,我们报告了在一系列连续的临床病例中使用QF-PCR的结果,并讨论了在不久的将来甚至可以替代所选样品上常规细胞遗传学分析的可能性。

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