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Design and validation of a pericentromeric BAC clone set aimed at improving diagnosis and phenotype prediction of supernumerary marker chromosomes

机译:设计和验证用于改善超数字标记染色体的诊断和表型预测的着丝粒BAC克隆集

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摘要

BackgroundSmall supernumerary marker chromosomes (sSMCs) are additional, structurally abnormal chromosomes, generally smaller than chromosome 20 of the same metaphase spread. Due to their small size, they are difficult to characterize by conventional cytogenetics alone. In regard to their clinical effects, sSMCs are a heterogeneous group: in particular, sSMCs containing pericentromeric euchromatin are likely to be associated with abnormal outcomes, although exceptions have been reported. To improve characterization of the genetic content of sSMCs, several approaches might be applied based on different molecular and molecular-cytogenetic assays, e.g., fluorescent in situ hybridization (FISH), array-based comparative genomic hybridization (array CGH), and multiplex ligation-dependent probe amplification (MLPA).To provide a complementary tool for the characterization of sSMCs, we constructed and validated a new, FISH-based, pericentromeric Bacterial Artificial Chromosome (BAC) clone set that with a high resolution spans the most proximal euchromatic sequences of all human chromosome arms, excluding the acrocentric short arms.
机译:背景技术小数目标记染色体(sSMCs)是其他结构异常的染色体,通常小于同一中期扩散的20号染色体。由于它们的体积小,它们难以仅通过常规细胞遗传学来表征。就其临床效果而言,sSMCs是一个异质性的群体:特别是,尽管有报道报道例外,但含有周围着丝粒常染色质的sSMCs可能与异常结果相关。为了改善sSMC遗传成分的特征,可以基于不同的分子和分子细胞遗传学检测方法,例如荧光原位杂交(FISH),基于阵列的比较基因组杂交(阵列CGH)和多重连接-依赖探针扩增(MLPA)。为提供表征sSMC的辅助工具,我们构建并验证了一种新的基于FISH的,以着丝粒为中心的细菌人工染色体(BAC)克隆集,该克隆集具有很高的分辨率,涵盖了所有人类染色体臂,不包括近端短臂。

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