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首页> 外文期刊>Molecular medicine reports >Rapid diagnosis of aneuploidy in chromosomes 13, 18, 21, X and y by quantitative fluorescence-PCR combined with short tandem repeat and fluorescence-labeled homologous gene quantitative-PCR using 4-color fluorescently labeled universal primers
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Rapid diagnosis of aneuploidy in chromosomes 13, 18, 21, X and y by quantitative fluorescence-PCR combined with short tandem repeat and fluorescence-labeled homologous gene quantitative-PCR using 4-color fluorescently labeled universal primers

机译:通过定量荧光PCR与短串联重复序列结合以及使用4色荧光标记通用引物的荧光标记同源基因定量PCR快速诊断13、18、21,X和y染色体上的非整倍性

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摘要

The present study aimed to develop a rapid diagnostic test of aneuploidy in chromosomes 13, 18, 21, X and Y through a program combining short tandem repeat (STR) typing with fluorescence-labeled homologous gene quantitative-polymerase chain reaction (fHGQ-PCR), which avoids misjudgment risks by using one method alone. Furthermore, fluorescently labeled universal primers not only ensure the accuracy of the results but also reduces the cost of fluorescent labels. The verification of DNA extracted from samples confirmed by karyotype analysis with quantitative fluorescence (QF)-PCR shows that the results obtained using the QF-PCR program are consistent with the results of karyotype analysis in rapidly diagnosing the aneuploidy of chromosomes 13, 18, 21, X and Y.
机译:本研究旨在通过结合短串联重复序列(STR)与荧光标记的同源基因定量聚合酶链反应(fHGQ-PCR)的程序,开发13、18、21,X和Y染色体非整倍性的快速诊断测试,这可以避免仅通过一种方法就可以判断错误的风险。此外,荧光标记的通用引物不仅确保结果的准确性,而且降低了荧光标记的成本。通过定量荧光(QF)-PCR进行核型分析确认的从样品中提取的DNA的验证表明,使用QF-PCR程序获得的结果与快速诊断13、18、21号染色体的非整倍性的核型分析结果一致,X和Y。

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