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首页> 外文期刊>The Journal of molecular diagnostics: JMD >Detection of chromosome aneuploidies in chorionic villus samples by multiplex ligation-dependent probe amplification.
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Detection of chromosome aneuploidies in chorionic villus samples by multiplex ligation-dependent probe amplification.

机译:通过多重连接依赖探针扩增检测绒毛膜绒毛样品中的染色体非整倍性。

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The objective of this study was to examine the suitability of multiplex ligation-dependent probe amplification (MLPA) in chorionic villus samples as a replacement for traditional karyotyping for the detection of (an)euploidies of chromosomes 21, 18, 13, X, and Y. Chorionic villus samples were diagnosed by traditional karyotyping using short-term cultures (STC) and long-term cultures (LTC), and by MLPA using kit P095. DNA was extracted after digestion of whole villi with proteinase K and/or trypsin and collagenase. Different cell-dissociation procedures were tested to obtain MLPA results representative of the cytotrophoblast layer and the mesenchymal core. Over 95% of the MLPA results were in concordance with the traditional karyotyping of STC and LTC. Traditional karyotyping revealed seven mosaics. After digestion of whole villi with proteinase K, only abnormal cell lines confined to the STC gave rise to abnormal MLPA results. In one sample, the complete discrepancy between STC and LTC was resolved after enzymatic dissociation of cells from the cytotrophoblast layer and the mesenchymal core. MLPA in chorionic villus samples was found to be a reliable test for the detection of (an)euploidies of chromosomes 21, 18, 13, X, and Y. Whole villi digestion with proteinase K resulted in the over-representation of cytotrophoblasts in the DNA pool. To obtain MLPA results representative for STC and LTC, enzymatic dissociation of cells from the cytotrophoblast layer and mesenchymal core is required.
机译:这项研究的目的是检查绒毛膜绒毛样品中多重连接依赖性探针扩增(MLPA)的适用性,以取代传统的核型分析方法,用于检测21、18、13,X和Y染色体的整倍性。绒毛膜绒毛样品通过使用短期培养物(STC)和长期培养物(LTC)的传统核型分析以及使用试剂盒P095的MLPA诊断。用蛋白酶K和/或胰蛋白酶和胶原酶消化整个绒毛后,提取DNA。测试了不同的细胞解离程序以获得代表细胞滋养层和间充质核心的MLPA结果。 MLPA结果的95%以上与STC和LTC的传统核型分析一致。传统的核型分析显示了七个镶嵌图。用蛋白酶K消化整个绒毛后,只有限于STC的异常细胞系才会导致MLPA结果异常。在一个样品中,从细胞滋养层和间充质核心中酶解离细胞后,STC和LTC之间的完全差异得以解决。发现绒毛膜绒毛样本中的MLPA是检测21、18、13,X和Y染色体正整倍体的可靠测试。用蛋白酶K进行的整个绒毛消化导致DNA中的细胞滋养层过度表达池。为了获得代表STC和LTC的MLPA结果,需要将细胞从滋养层和间充质核心中酶解离。

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