Analysis of quality metrics in comprehensive cancer genomic profiling using a dual DNA–RNA panel

IF 1.7 Q3 MEDICAL LABORATORY TECHNOLOGY Practical Laboratory Medicine Pub Date : 2024-02-15 DOI:10.1016/j.plabm.2024.e00368
Kousuke Watanabe , Shinji Kohsaka , Kenji Tatsuno , Aya Shinozaki-Ushiku , Hideaki Isago , Hidenori Kage , Tetsuo Ushiku , Hiroyuki Aburatani , Hiroyuki Mano , Katsutoshi Oda
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Abstract

Background

The nucleic acid quality from formalin-fixed paraffin-embedded (FFPE) tumor vary among samples, resulting in substantial variability in the quality of comprehensive cancer genomic profiling tests. The objective of the study is to investigate how nucleic acid quality affects sequencing quality. We also examined the variations in nucleic acid quality among different hospitals or cancer types.

Methods

Three nucleic acid quality metrics (ddCq, Q-value, and DV200) and five sequencing quality metrics (on-target rate, mean depth, coverage uniformity, target exon coverage, and coverage of the housekeeping gene) were examined using 585 samples from the Todai OncoPanel, a dual DNA–RNA panel.

Results

In the DNA panel, ddCq served as an indicator of sequencing depth and Q-value reflected the uniformity of sequencing across different regions. It was essential to have favorable values not only for ddCq but also for Q-value to obtain ideal sequencing results. For the RNA panel, DV200 proved to be a valuable metric for assessing the coverage of the housekeeping genes. Significant inter-hospital differences were observed for DNA quality (ddCq and Q-value), but not for RNA quality (DV200). Differences were also observed among cancer types, with Q-value being the lowest in lung and the highest in cervix, while DV200 was the highest in lung and the lowest in bowel.

Conclusions

We demonstrated distinct characteristics and high predictive performances of ddCq, Q-value, and DV200. Variations were observed in the nucleic acid quality across hospitals and cancer types. Further study is warranted on preanalytical factors in comprehensive cancer genomic profiling tests.

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利用双 DNA-RNA 面板分析癌症基因组综合分析的质量指标
背景福尔马林固定石蜡包埋(FFPE)肿瘤的核酸质量因样本而异,导致癌症基因组综合分析测试的质量存在很大差异。本研究旨在探讨核酸质量如何影响测序质量。我们还研究了核酸质量在不同医院或不同癌症类型之间的差异。方法使用 585 份来自 Todai OncoPanel(DNA-RNA 双面板)的样本,检测了三个核酸质量指标(ddCq、Q 值和 DV200)和五个测序质量指标(靶上率、平均深度、覆盖均匀性、靶外显子覆盖率和看家基因覆盖率)。结果 在 DNA 面板中,ddCq 是测序深度的指标,Q 值反映了不同区域测序的均匀性。要获得理想的测序结果,不仅要有良好的 ddCq 值,还要有良好的 Q 值。对于 RNA 面板,DV200 被证明是评估看家基因覆盖率的重要指标。在DNA质量(ddCq和Q值)方面观察到了医院间的显著差异,但在RNA质量(DV200)方面没有观察到显著差异。癌症类型之间也存在差异,肺癌的 Q 值最低,宫颈癌的 Q 值最高,而肺癌的 DV200 最高,肠癌的 DV200 最低。不同医院和癌症类型的核酸质量存在差异。有必要进一步研究癌症基因组图谱综合测试的分析前因素。
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来源期刊
Practical Laboratory Medicine
Practical Laboratory Medicine Health Professions-Radiological and Ultrasound Technology
CiteScore
3.50
自引率
0.00%
发文量
40
审稿时长
7 weeks
期刊介绍: Practical Laboratory Medicine is a high-quality, peer-reviewed, international open-access journal publishing original research, new methods and critical evaluations, case reports and short papers in the fields of clinical chemistry and laboratory medicine. The objective of the journal is to provide practical information of immediate relevance to workers in clinical laboratories. The primary scope of the journal covers clinical chemistry, hematology, molecular biology and genetics relevant to laboratory medicine, microbiology, immunology, therapeutic drug monitoring and toxicology, laboratory management and informatics. We welcome papers which describe critical evaluations of biomarkers and their role in the diagnosis and treatment of clinically significant disease, validation of commercial and in-house IVD methods, method comparisons, interference reports, the development of new reagents and reference materials, reference range studies and regulatory compliance reports. Manuscripts describing the development of new methods applicable to laboratory medicine (including point-of-care testing) are particularly encouraged, even if preliminary or small scale.
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