DNA methylation biomarkers distinguishing early-stage prostate cancer from benign prostatic hyperplasia

IF 2.7 2区 医学 Q2 UROLOGY & NEPHROLOGY Prostate International Pub Date : 2023-06-01 DOI:10.1016/j.prnil.2023.01.001
Stephanie S. Kim , Seung Cho Lee , Bumjin Lim , Seung-Ho Shin , Mee Young Kim , Sol-Yi Kim , Hyeyeun Lim , Clémentine Charton , Dongho Shin , Hyong Woo Moon , Jinho Kim , Donghyun Park , Woong-Yang Park , Ji Youl Lee
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Abstract

Background

DNA methylation markers are considered robust diagnostic features in various cancer types, as epigenetic marks are commonly altered during cancer progression. Differentiation between benign prostatic hyperplasia (BPH) and early-stage prostate cancer (PCa) is clinically difficult, relying on the information of the patient's symptoms or levels of prostate-specific antigen.

Methods

A total of 42 PCa patients and 11 BPH patients were recruited. Genomic DNA was purified from tissues and used for the library preparation of the target-enriched methylome with enzymatic conversion and a Twist 85 Mbp EM-seq panel. Paired-end sequencing (150 bp) was performed using NovaSeq 6000 or NextSeq 550. After quality control, including adapter trimming and de-duplication of raw sequencing data, differential methylation patterns were analyzed between the BPH and PCa groups.

Results

We report DNA methylation patterns existing between BPH and PCa. The major finding is that broad hypermethylation occurred at genic loci in PCa tissues as compared to the BPH. Gene ontology analysis suggested that hypermethylation of genic loci involved in chromatin and transcriptional regulation is involved in cancer progression. We also compared PCa tissues with high Gleason scores to tissues with low Gleason scores. The high-Gleason PCa tissues showed hundreds of focal differentially methylated CpG sites corresponding to genes functioning in cancer cell proliferation or metastasis. This suggests that dissecting early-to-advanced-grade cancer stages requires an in-depth analysis of differential methylation at the single CpG site level.

Conclusions

Our study reports that enzymatic methylome sequencing data can be used to distinguish PCa from BPH and advanced PCa from early-stage PCa. The stage-specific methylation patterns in this study will be valuable resources for diagnostic purposes as well as further development of liquid biopsy approaches for the early detection of PCa.

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区分早期前列腺癌症和良性前列腺增生的DNA甲基化生物标志物
背景DNA甲基化标记物被认为是各种癌症类型的强大诊断特征,因为表观遗传标记物通常在癌症进展过程中发生改变。根据患者症状或前列腺特异性抗原水平的信息,在临床上很难区分良性前列腺增生症(BPH)和早期前列腺癌症(PCa)。方法对42例前列腺增生症患者和11例前列腺增生患者进行临床调查。从组织中纯化基因组DNA,并用于文库制备具有酶转化和Twist 85Mbp-EM-seq面板的靶富集甲基组。使用NovaSeq 6000或NextSeq 550进行配对末端测序(150bp)。经过质量控制,包括适配器修剪和原始测序数据的重复消除,分析了前列腺增生组和前列腺癌组之间的差异甲基化模式。结果我们报道了前列腺增生和前列腺癌之间存在的DNA甲基化模式。主要发现是,与前列腺增生相比,前列腺癌组织中的基因座发生了广泛的超甲基化。基因本体论分析表明,参与染色质和转录调控的基因位点的高甲基化参与了癌症的进展。我们还比较了Gleason评分高的前列腺癌组织和Gleason分数低的组织。高Gleason PCa组织显示数百个与癌症细胞增殖或转移功能基因相对应的局灶性差异甲基化CpG位点。这表明,解剖早期到晚期癌症阶段需要在单个CpG位点水平上对差异甲基化进行深入分析。结论我们的研究报告称,酶甲基组测序数据可用于区分前列腺增生和前列腺增生,以及晚期前列腺增生和早期前列腺增生。本研究中的阶段特异性甲基化模式将是诊断目的以及进一步开发早期检测前列腺癌的液体活检方法的宝贵资源。
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来源期刊
Prostate International
Prostate International Medicine-Urology
CiteScore
4.40
自引率
26.70%
发文量
40
审稿时长
35 days
期刊介绍: Prostate International (Prostate Int, PI), the official English-language journal of Asian Pacific Prostate Society (APPS), is an international peer-reviewed academic journal dedicated to basic and clinical studies on prostate cancer, benign prostatic hyperplasia, prostatitis, and ...
期刊最新文献
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