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通过显微切割技术在产前诊断中对标记染色体进行完整而精确的特征描述。

Complete and precise characterization of marker chromosomes by application of microdissection in prenatal diagnosis.

作者信息

Müller-Navia J, Nebel A, Schleiermacher E

机构信息

Institut für Anthropologie, Universität Mainz, Germany.

出版信息

Hum Genet. 1995 Dec;96(6):661-7. doi: 10.1007/BF00210295.

Abstract

A straightforward and extremely efficient reverse chromosome painting technique is described which allows the rapid and unequivocal identification of any cytogenetically unclassifiable chromosome rearrangement. This procedure is used to determine the origin of unknown marker chromosomes found at prenatal diagnosis. After microdissection of the marker chromosome and amplification of the dissected fragment by a degenerate oligonucleotide-primed polymerase chain reaction (DOP-PCR), fluorescence in situ hybridization (FISH) to aberrant and normal metaphase chromosomes with the marker-derived probe pool is performed. With this strategy, marker chromosomes present in amniotic fluid samples were successfully identified in three cases. The origin of the supernumerary markers was ascertained as deriving from 3p(p12-cen), 18p(pter-cen) and 9p(p12-cen), respectively. Since a specific FISH signal on chromosomes can be obtained within 2 working days using a probe generated without any pretreatment from one chromosomal fragment only and without additional image processing devices, this technique is considered to be highly suitable for routine application in pre- and postnatal cytogenetic analysis.

摘要

本文描述了一种简单且极其高效的反向染色体描绘技术,该技术可快速明确地识别任何细胞遗传学上无法分类的染色体重排。此程序用于确定产前诊断时发现的未知标记染色体的起源。在对标记染色体进行显微切割,并通过简并寡核苷酸引物聚合酶链反应(DOP-PCR)扩增切割片段后,使用标记物衍生的探针池对异常和正常中期染色体进行荧光原位杂交(FISH)。采用这种策略,在三例羊水样本中成功鉴定出了标记染色体。额外标记物的起源分别确定为源自3p(p12-着丝粒)、18p(端粒-着丝粒)和9p(p12-着丝粒)。由于仅使用一个未经任何预处理的染色体片段生成的探针,无需额外图像处理设备,在2个工作日内即可在染色体上获得特定的FISH信号,因此该技术被认为非常适合在产前和产后细胞遗传学分析中常规应用。

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