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

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

doi:10.1016/j.prnil.2023.01.001

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

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

Department of Urology

Research output: Contribution to journal › Article › peer-review

11 Scopus citations

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.

Original language	English
Pages (from-to)	113-121
Number of pages	9
Journal	Prostate International
Volume	11
Issue number	2
DOIs	https://doi.org/10.1016/j.prnil.2023.01.001
State	Published - Jun 2023

Bibliographical note

Publisher Copyright:
© 2023

Keywords

Benign prostatic hyperplasia
Biomarkers
Cancer diagnosis
DNA methylation
Enzymatic conversion
Gleason score
Prostate cancer
Target enrichment sequencing

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

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10.1016/j.prnil.2023.01.001

Cite this

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title = "DNA methylation biomarkers distinguishing early-stage prostate cancer from benign prostatic hyperplasia",

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.",

keywords = "Benign prostatic hyperplasia, Biomarkers, Cancer diagnosis, DNA methylation, Enzymatic conversion, Gleason score, Prostate cancer, Target enrichment sequencing",

author = "Kim, {Stephanie S.} and Lee, {Seung Cho} and Bumjin Lim and Shin, {Seung Ho} and Kim, {Mee Young} and Kim, {Sol Yi} and Hyeyeun Lim and Cl{\'e}mentine Charton and Dongho Shin and Moon, {Hyong Woo} and Jinho Kim and Donghyun Park and Park, {Woong Yang} and Lee, {Ji Youl}",

note = "Publisher Copyright: {\textcopyright} 2023",

year = "2023",

month = jun,

doi = "10.1016/j.prnil.2023.01.001",

language = "English",

volume = "11",

pages = "113--121",

journal = "Prostate International",

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publisher = "Elsevier B.V.",

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TY - JOUR

T1 - DNA methylation biomarkers distinguishing early-stage prostate cancer from benign prostatic hyperplasia

AU - Kim, Stephanie S.

AU - Lee, Seung Cho

AU - Lim, Bumjin

AU - Shin, Seung Ho

AU - Kim, Mee Young

AU - Kim, Sol Yi

AU - Lim, Hyeyeun

AU - Charton, Clémentine

AU - Shin, Dongho

AU - Moon, Hyong Woo

AU - Kim, Jinho

AU - Park, Donghyun

AU - Park, Woong Yang

AU - Lee, Ji Youl

PY - 2023/6

Y1 - 2023/6

N2 - 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.

AB - 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.

KW - Benign prostatic hyperplasia

KW - Biomarkers

KW - Cancer diagnosis

KW - DNA methylation

KW - Enzymatic conversion

KW - Gleason score

KW - Prostate cancer

KW - Target enrichment sequencing

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U2 - 10.1016/j.prnil.2023.01.001

DO - 10.1016/j.prnil.2023.01.001

M3 - Article

AN - SCOPUS:85150345751

SN - 2287-8882

VL - 11

SP - 113

EP - 121

JO - Prostate International

JF - Prostate International

IS - 2

ER -

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

Abstract

Bibliographical note

Keywords

UN SDGs

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