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Deep sequencing of target linkage assay-identified regions in familial breast cancer: methods, analysis pipeline and troubleshooting

机译:靶点连锁测定法鉴定的家族性乳腺癌区域的深度测序:方法,分析流程和故障排除

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摘要

BACKGROUND: The classical candidate-gene approach has failed to identify novel breast cancer susceptibility genes. Nowadays, massive parallel sequencing technology allows the development of studies unaffordable a few years ago. However, analysis protocols are not yet sufficiently developed to extract all information from the huge amount of data obtained. METHODOLOGY/PRINCIPAL FINDINGS: In this study, we performed high throughput sequencing in two regions located on chromosomes 3 and 6, recently identified by linkage studies by our group as candidate regions for harbouring breast cancer susceptibility genes. In order to enrich for the coding regions of all described genes located in both candidate regions, a hybrid-selection method on tiling microarrays was performed. CONCLUSIONS/SIGNIFICANCE: We developed an analysis pipeline based on SOAP aligner to identify candidate variants with a high real positive confirmation rate (0.89), with which we identified eight variants considered candidates for functional studies. The results suggest that the present strategy might be a valid second step for identifying high penetrance genes.
机译:背景:经典的候选基因方法未能鉴定出新型的乳腺癌易感基因。如今,大规模的并行测序技术使几年前无法负担的研究发展成为可能。但是,分析协议尚未得到充分开发,无法从获得的大量数据中提取所有信息。方法/主要发现:在这项研究中,我们在3号和6号染色体上的两个区域进行了高通量测序,最近我们小组通过连锁研究将其鉴定为具有乳腺癌易感基因的候选区域。为了丰富位于两个候选区域中的所有描述基因的编码区域,在平铺微阵列上进行了杂交选择方法。结论/意义:我们开发了一种基于SOAP aligner的分析流程,以鉴定具有较高真实肯定确认率(0.89)的候选变体,从而确定了八种被视为功能研究候选变体。结果表明,本策略可能是鉴定高外显率基因的有效第二步。

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