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A sequential methodology for the rapid identification and characterization of breast cancer-associated functional SNPs

机译:一种顺序方法,用于快速鉴定和表征乳腺癌相关功能SNP

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GWAS cannot identify functional SNPs (fSNP) from disease-associated SNPs in linkage disequilibrium (LD). Here, we report developing three sequential methodologies including Reel-seq (Regulatory element-sequencing) to identify fSNPs in a high-throughput fashion, SDCP-MS (SNP-specific DNA competition pulldown-mass spectrometry) to identify fSNP-bound proteins and AIDP-Wb (allele-imbalanced DNA pulldown-Western blot) to detect allele-specific protein:fSNP binding. We first apply Reel-seq to screen a library containing 4316 breast cancer-associated SNPs and identify 521 candidate fSNPs. As proof of principle, we verify candidate fSNPs on three well-characterized loci: FGFR2, MAP3K1 and BABAM1. Next, using SDCP-MS and AIDP-Wb, we rapidly identify multiple regulatory factors that specifically bind in an allele-imbalanced manner to the fSNPs on the FGFR2 locus. We finally demonstrate that the factors identified by SDCP-MS can regulate risk gene expression. These data suggest that the sequential application of Reel-seq, SDCP-MS, and AIDP-Wb can greatly help to translate large sets of GWAS data into biologically relevant information.
机译:Gwas不能在连杆不平衡(LD)中的疾病相关的SNP中识别功能性SNPS(FSNP)。在这里,我们报告了三种顺序方法,包括reel-seq(调节元素测序),以鉴定高通量时尚,SDCP-MS(SNP特异性DNA竞争下式 - 质谱)识别FSNP,以鉴定FSNP结合的蛋白质和AIDP -WB(等位基因 - 不平衡DNA下拉 - Western印迹)检测等位基因特异性蛋白质:FSNP结合。我们首先应用Reel-SEQ以筛选包含4316例乳腺癌相关的SNP的库,并确定521个候选FSNP。作为原则的证据,我们验证了三个特征的基因座的候选FSNP:FGFR2,MAP3K1和Babam1。接下来,使用SDCP-MS和AIDP-WB,我们迅速识别多种调节因子,该因素以等位基因 - 不平衡方式特异性地与FGFR2基因座上的FSNP结合。我们终于证明了SDCP-MS鉴定的因素可以调节风险基因表达。这些数据表明,Reel-SEQ,SDCP-MS和AIDP-WB的顺序应用可以大大帮助将大型GWAS数据转化为生物学相关信息。

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