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高通量测序分析人类乳腺癌细胞和正常细胞中串联 3'UTR 的差异全基因组图谱。

Differential genome-wide profiling of tandem 3' UTRs among human breast cancer and normal cells by high-throughput sequencing.

机构信息

State Key Laboratory for Biocontrol, Guangdong Province Key Laboratory of Pharmaceutical Functional Genes, Department of Biochemistry, College of Life Sciences, Sun Yat-sen University, Higher Education Mega Center, Guangzhou 510006, P.R. China.

出版信息

Genome Res. 2011 May;21(5):741-7. doi: 10.1101/gr.115295.110. Epub 2011 Apr 7.

Abstract

Tandem 3' UTRs produced by alternative polyadenylation (APA) play an important role in gene expression by impacting mRNA stability, translation, and translocation in cells. Several studies have investigated APA site switching in various physiological states; nevertheless, they only focused on either the genes with two known APA sites or several candidate genes. Here, we developed a strategy to study APA sites in a genome-wide fashion with second-generation sequencing technology which could not only identify new polyadenylation sites but also analyze the APA site switching of all genes, especially those with more than two APA sites. We used this strategy to explore the profiling of APA sites in two human breast cancer cell lines, MCF7 and MB231, and one cultured mammary epithelial cell line, MCF10A. More than half of the identified polyadenylation sites are not included in human poly(A) databases. While MCF7 showed shortening 3' UTRs, more genes in MB231 switched to distal poly(A) sites. Several gene ontology (GO) terms and pathways were enriched in the list of genes with switched APA sites, including cell cycle, apoptosis, and metabolism. These results suggest a more complex regulation of APA sites in cancer cells than previously thought. In short, our novel unbiased method can be a powerful approach to cost-effectively investigate the complex mechanism of 3' UTR switching in a genome-wide fashion among various physiological processes and diseases.

摘要

串联 3'UTR 通过可变多聚腺苷酸化(APA)产生,通过影响细胞中的 mRNA 稳定性、翻译和易位,在基因表达中发挥重要作用。有几项研究调查了各种生理状态下的 APA 位点转换;然而,它们仅关注具有两个已知 APA 位点的基因或几个候选基因。在这里,我们开发了一种使用第二代测序技术在全基因组范围内研究 APA 位点的策略,该策略不仅可以识别新的多聚腺苷酸化位点,还可以分析所有基因的 APA 位点转换,特别是那些具有两个以上 APA 位点的基因。我们使用这种策略来探索两种人乳腺癌细胞系 MCF7 和 MB231 以及一种培养的乳腺上皮细胞系 MCF10A 中的 APA 位点谱。所鉴定的多聚腺苷酸化位点中有一半以上不包含在人类 poly(A) 数据库中。虽然 MCF7 显示 3'UTR 缩短,但 MB231 中更多的基因切换到远端 poly(A) 位点。在 APA 位点切换的基因列表中富集了几个基因本体论 (GO) 术语和途径,包括细胞周期、细胞凋亡和代谢。这些结果表明,癌症细胞中 APA 位点的调控比以前想象的更为复杂。简而言之,我们的新的无偏方法可以成为一种有效的方法,以具有成本效益的方式在各种生理过程和疾病中在全基因组范围内研究 3'UTR 切换的复杂机制。

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