{"title":"446: crispr - snp -seq鉴定了前列腺癌的调控位点","authors":"Yijun Tian, Jong-A Park, Liang Wang","doi":"10.1158/1538-7445.AM2021-446","DOIUrl":null,"url":null,"abstract":"Introduction: Genome-wide association studies (GWAS) along with expression quantitative trait loci (eQTL) have identified hundreds of genetic variants and target genes in prostate cancer (prCa). Although genetic predisposition has mainly been described in prostate cancer (PrCa), functional characterization of these risk loci remains a challenge. Methods: Low multiplicity of infection creates single lentiviral integrated cell population, which enable us to evaluate biological significance of steric hindrance at certain SNP sites in large scale. To screen for regulatory SNP, we designed a guide RNA library to target 2166 potential functional SNP sites with CRISPOR software. We performed negative screening in dCas9-KRAB stable prostate cell lines and applied RIGOR program to discover the SNPs that are essential for cell proliferation. We further validated regulatory role of selected SNPs using luciferase reporter assay, ChIP-qPCR and CRISPR-based SNP editing in prostate cells. Results: After gRNA interfering for 21 days, we performed RIGOR analysis and identified 153 proliferation-essential SNPs, covered by one or multiple prostate cancer cell lines. Intersection analysis showed that these SNPs tended to reside in 59-UTR and intron regions. To characterize regulatory role of these SNPs, we performed functional analysis in a SNP rs60 since prostate cells containing guide RNAs targeting rs60 were significantly depleted (FDR Conclusion: CRISPRi-SNPs-seq is a powerful screening tool to identify regulatory SNPs essential for cell proliferation. In combination with in-depth functional assays, the technology will facilitate discovery of regulatory variants and their genes responsible for disease risk. Citation Format: Yijun Tian, Jong A. Park, Liang Wang. CRISPRi-SNPs-seq identified regulatory loci conferring prostate cancer [abstract]. In: Proceedings of the American Association for Cancer Research Annual Meeting 2021; 2021 Apr 10-15 and May 17-21. Philadelphia (PA): AACR; Cancer Res 2021;81(13_Suppl):Abstract nr 446.","PeriodicalId":10518,"journal":{"name":"Clinical Research (Excluding Clinical Trials)","volume":"18 1","pages":""},"PeriodicalIF":0.0000,"publicationDate":"2021-07-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":"{\"title\":\"Abstract 446: CRISPRi-SNPs-seq identified regulatory loci conferring prostate cancer\",\"authors\":\"Yijun Tian, Jong-A Park, Liang Wang\",\"doi\":\"10.1158/1538-7445.AM2021-446\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"Introduction: Genome-wide association studies (GWAS) along with expression quantitative trait loci (eQTL) have identified hundreds of genetic variants and target genes in prostate cancer (prCa). Although genetic predisposition has mainly been described in prostate cancer (PrCa), functional characterization of these risk loci remains a challenge. Methods: Low multiplicity of infection creates single lentiviral integrated cell population, which enable us to evaluate biological significance of steric hindrance at certain SNP sites in large scale. To screen for regulatory SNP, we designed a guide RNA library to target 2166 potential functional SNP sites with CRISPOR software. We performed negative screening in dCas9-KRAB stable prostate cell lines and applied RIGOR program to discover the SNPs that are essential for cell proliferation. We further validated regulatory role of selected SNPs using luciferase reporter assay, ChIP-qPCR and CRISPR-based SNP editing in prostate cells. Results: After gRNA interfering for 21 days, we performed RIGOR analysis and identified 153 proliferation-essential SNPs, covered by one or multiple prostate cancer cell lines. Intersection analysis showed that these SNPs tended to reside in 59-UTR and intron regions. To characterize regulatory role of these SNPs, we performed functional analysis in a SNP rs60 since prostate cells containing guide RNAs targeting rs60 were significantly depleted (FDR Conclusion: CRISPRi-SNPs-seq is a powerful screening tool to identify regulatory SNPs essential for cell proliferation. In combination with in-depth functional assays, the technology will facilitate discovery of regulatory variants and their genes responsible for disease risk. Citation Format: Yijun Tian, Jong A. Park, Liang Wang. CRISPRi-SNPs-seq identified regulatory loci conferring prostate cancer [abstract]. In: Proceedings of the American Association for Cancer Research Annual Meeting 2021; 2021 Apr 10-15 and May 17-21. 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引用次数: 0
摘要
全基因组关联研究(GWAS)和表达数量性状位点(eQTL)已经在前列腺癌(prCa)中发现了数百种遗传变异和靶基因。虽然遗传易感性主要描述在前列腺癌(PrCa),功能表征这些风险位点仍然是一个挑战。方法:低感染的多重性形成单一的慢病毒整合细胞群,这使我们能够大规模地评估某些SNP位点的空间阻滞性的生物学意义。为了筛选调控SNP,我们设计了一个引导RNA文库,利用CRISPOR软件靶向2166个潜在的功能SNP位点。我们对dCas9-KRAB稳定的前列腺细胞系进行阴性筛选,并应用RIGOR程序发现细胞增殖所必需的snp。我们在前列腺细胞中使用荧光素酶报告基因检测、ChIP-qPCR和基于crispr的SNP编辑进一步验证了所选SNP的调节作用。结果:在gRNA干扰21天后,我们进行了严格分析,鉴定出153个增殖必需snp,覆盖在一个或多个前列腺癌细胞系中。交叉分析表明,这些snp倾向于位于59-UTR和内含子区域。为了表征这些SNP的调控作用,我们对SNP rs60进行了功能分析,因为含有靶向rs60的引导rna的前列腺细胞显着耗尽(FDR结论:crispr -SNP -seq是鉴定细胞增殖必需的调控SNP的强大筛选工具。结合深入的功能分析,该技术将有助于发现调节变异及其与疾病风险相关的基因。引用格式:田义军,朴钟a,王亮。crispr - snp -seq鉴定了前列腺癌的调控位点[摘要]。见:美国癌症研究协会2021年年会论文集;2021年4月10日至15日和5月17日至21日。费城(PA): AACR;癌症杂志,2021;81(13 -增刊):摘要第446期。
Abstract 446: CRISPRi-SNPs-seq identified regulatory loci conferring prostate cancer
Introduction: Genome-wide association studies (GWAS) along with expression quantitative trait loci (eQTL) have identified hundreds of genetic variants and target genes in prostate cancer (prCa). Although genetic predisposition has mainly been described in prostate cancer (PrCa), functional characterization of these risk loci remains a challenge. Methods: Low multiplicity of infection creates single lentiviral integrated cell population, which enable us to evaluate biological significance of steric hindrance at certain SNP sites in large scale. To screen for regulatory SNP, we designed a guide RNA library to target 2166 potential functional SNP sites with CRISPOR software. We performed negative screening in dCas9-KRAB stable prostate cell lines and applied RIGOR program to discover the SNPs that are essential for cell proliferation. We further validated regulatory role of selected SNPs using luciferase reporter assay, ChIP-qPCR and CRISPR-based SNP editing in prostate cells. Results: After gRNA interfering for 21 days, we performed RIGOR analysis and identified 153 proliferation-essential SNPs, covered by one or multiple prostate cancer cell lines. Intersection analysis showed that these SNPs tended to reside in 59-UTR and intron regions. To characterize regulatory role of these SNPs, we performed functional analysis in a SNP rs60 since prostate cells containing guide RNAs targeting rs60 were significantly depleted (FDR Conclusion: CRISPRi-SNPs-seq is a powerful screening tool to identify regulatory SNPs essential for cell proliferation. In combination with in-depth functional assays, the technology will facilitate discovery of regulatory variants and their genes responsible for disease risk. Citation Format: Yijun Tian, Jong A. Park, Liang Wang. CRISPRi-SNPs-seq identified regulatory loci conferring prostate cancer [abstract]. In: Proceedings of the American Association for Cancer Research Annual Meeting 2021; 2021 Apr 10-15 and May 17-21. Philadelphia (PA): AACR; Cancer Res 2021;81(13_Suppl):Abstract nr 446.
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