Challenges in next generation sequencing of homology recombination repair genomic variants in prostate cancer: A nationwide survey and calibration project in China

BACKGROUND: Homologous Recombination Repair (HRR) is the most reliable and important signaling pathway for repairing DNA damage. We initiated a calibration project to better understand the NGS landscape for HRR gene testing in China, provide indications for testing standardization, and guide clinica...

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Autores principales: Wu, Huanwen, Zhou, Liqun, Zhou, Xiaoyan, Wei, Qiang, Ouyang, Nengtai, Shao, Jianyong, Huang, Jian, Liang, Zhiyong
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Asian Pacific Prostate Society 2022
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9747577/
https://www.ncbi.nlm.nih.gov/pubmed/36570645
http://dx.doi.org/10.1016/j.prnil.2022.07.002
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author Wu, Huanwen
Zhou, Liqun
Zhou, Xiaoyan
Wei, Qiang
Ouyang, Nengtai
Shao, Jianyong
Huang, Jian
Liang, Zhiyong
author_facet Wu, Huanwen
Zhou, Liqun
Zhou, Xiaoyan
Wei, Qiang
Ouyang, Nengtai
Shao, Jianyong
Huang, Jian
Liang, Zhiyong
author_sort Wu, Huanwen
collection PubMed
description BACKGROUND: Homologous Recombination Repair (HRR) is the most reliable and important signaling pathway for repairing DNA damage. We initiated a calibration project to better understand the NGS landscape for HRR gene testing in China, provide indications for testing standardization, and guide clinical practice. METHODS: A questionnaire was used to collect laboratory information, panel design for HRR gene testing, tissue sample test parameters, plasma ctDNA sample test parameters, and procedures for variant interpretation. The testing quality of the participating laboratories was further evaluated by external quality assessment (EQA), which provided 5 FFPE slices and 5 mimic ctDNA samples as standard references for evaluation. Test results and reports were collected to assess laboratory performance. RESULTS: Our results showed that different laboratories had significant differences in sequencing platforms, library construction technologies, genes in the testing panel, detectable mutation types, probe coverage regions, sequencing parameters, variants interpretation guidelines, and positive test rates. For the EQA test, the overall pass rate was about 60%. The average accuracy for tissue samples and ctDNA samples was 79.55% and 74.13%, respectively. It is worth noting that variants in tandem repetition regions and splice sites, and those with low allele frequency were more prone to misdetection. The most common reasons for misdetection were as follows: the testing panel did not cover the genes or the whole exon and splice sites of the genes; the variants were misclassified as benign or likely benign, and the variants failed the QC criteria. CONCLUSIONS: The discrepancies observed in our survey and EQA test affect the authenticity of HRR gene test results for prostate cancer, underlining the need to establish guidelines for HRR gene testing and variant interpretation in China, and to optimize HRR gene testing in clinical practice to improve management and patient care.
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spelling pubmed-97475772022-12-22 Challenges in next generation sequencing of homology recombination repair genomic variants in prostate cancer: A nationwide survey and calibration project in China Wu, Huanwen Zhou, Liqun Zhou, Xiaoyan Wei, Qiang Ouyang, Nengtai Shao, Jianyong Huang, Jian Liang, Zhiyong Prostate Int Research Article BACKGROUND: Homologous Recombination Repair (HRR) is the most reliable and important signaling pathway for repairing DNA damage. We initiated a calibration project to better understand the NGS landscape for HRR gene testing in China, provide indications for testing standardization, and guide clinical practice. METHODS: A questionnaire was used to collect laboratory information, panel design for HRR gene testing, tissue sample test parameters, plasma ctDNA sample test parameters, and procedures for variant interpretation. The testing quality of the participating laboratories was further evaluated by external quality assessment (EQA), which provided 5 FFPE slices and 5 mimic ctDNA samples as standard references for evaluation. Test results and reports were collected to assess laboratory performance. RESULTS: Our results showed that different laboratories had significant differences in sequencing platforms, library construction technologies, genes in the testing panel, detectable mutation types, probe coverage regions, sequencing parameters, variants interpretation guidelines, and positive test rates. For the EQA test, the overall pass rate was about 60%. The average accuracy for tissue samples and ctDNA samples was 79.55% and 74.13%, respectively. It is worth noting that variants in tandem repetition regions and splice sites, and those with low allele frequency were more prone to misdetection. The most common reasons for misdetection were as follows: the testing panel did not cover the genes or the whole exon and splice sites of the genes; the variants were misclassified as benign or likely benign, and the variants failed the QC criteria. CONCLUSIONS: The discrepancies observed in our survey and EQA test affect the authenticity of HRR gene test results for prostate cancer, underlining the need to establish guidelines for HRR gene testing and variant interpretation in China, and to optimize HRR gene testing in clinical practice to improve management and patient care. Asian Pacific Prostate Society 2022-12 2022-07-22 /pmc/articles/PMC9747577/ /pubmed/36570645 http://dx.doi.org/10.1016/j.prnil.2022.07.002 Text en © 2022 Asian Pacific Prostate Society. Publishing services by Elsevier B.V. https://creativecommons.org/licenses/by-nc-nd/4.0/This is an open access article under the CC BY-NC-ND license (http://creativecommons.org/licenses/by-nc-nd/4.0/).
spellingShingle Research Article
Wu, Huanwen
Zhou, Liqun
Zhou, Xiaoyan
Wei, Qiang
Ouyang, Nengtai
Shao, Jianyong
Huang, Jian
Liang, Zhiyong
Challenges in next generation sequencing of homology recombination repair genomic variants in prostate cancer: A nationwide survey and calibration project in China
title Challenges in next generation sequencing of homology recombination repair genomic variants in prostate cancer: A nationwide survey and calibration project in China
title_full Challenges in next generation sequencing of homology recombination repair genomic variants in prostate cancer: A nationwide survey and calibration project in China
title_fullStr Challenges in next generation sequencing of homology recombination repair genomic variants in prostate cancer: A nationwide survey and calibration project in China
title_full_unstemmed Challenges in next generation sequencing of homology recombination repair genomic variants in prostate cancer: A nationwide survey and calibration project in China
title_short Challenges in next generation sequencing of homology recombination repair genomic variants in prostate cancer: A nationwide survey and calibration project in China
title_sort challenges in next generation sequencing of homology recombination repair genomic variants in prostate cancer: a nationwide survey and calibration project in china
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9747577/
https://www.ncbi.nlm.nih.gov/pubmed/36570645
http://dx.doi.org/10.1016/j.prnil.2022.07.002
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