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首页> 外文期刊>The Journal of molecular diagnostics: JMD >Describing the Reportable Range Is Important for Reliable Treatment Decisions A Multiple Laboratory Study for Molecular Tumor Profiling Using Next-Generation Sequencing
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Describing the Reportable Range Is Important for Reliable Treatment Decisions A Multiple Laboratory Study for Molecular Tumor Profiling Using Next-Generation Sequencing

机译:描述可报告范围对于可靠的治疗决策对于使用下一代测序的分子肿瘤分析的多个实验室研究是重要的

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摘要

Because interpretation of next-generation sequencing (NGS) data remains challenging, optimization of the NGS process is needed to obtain correct sequencing results. Therefore, extensive validation and continuous monitoring of the quality is essential. NGS performance was compared with traditional detection methods and technical quality of nine NGS technologies was assessed. First, nine formalin-fixed, paraffin-embedded patient samples were analyzed by 114 laboratories by using different detection methods. No significant differences in performance were observed between analyses with NGS and traditional techniques. Second, two DNA control samples were analyzed for a selected number of variants by 26 participants with the use of nine different NGS technologies. Quality control metrics were analyzed from raw data files and a survey about routine procedures. Results showed large differences in coverages, but observed variant allele frequencies in raw data files were in line with predefined variant allele frequencies. Many false negative results were found because of low-quality regions, which were not reported as such. It is recommended to disclose the reportable range, the fraction of targeted genomic regions for which calls of acceptable quality can be generated, to avoid any errors in therapy decisions. NGS can be a reliable technique, only if essential quality control during analysis is applied and reported.
机译:因为下一代测序(NGS)数据的解释仍然有挑战性,所以需要优化NGS过程以获得正确的测序结果。因此,广泛的验证和对质量的持续监测至关重要。 NGS性能与传统的检测方法进行了比较,评估了九种NGS技术的技术质量。首先,通过使用不同的检测方法,通过114实验室分析九种福尔马林固定的石蜡嵌入的患者样品。在具有NGS和传统技术的分析之间没有观察到性能显着差异。其次,通过使用九种不同的NGS技术分析26名参与者的选定数量的变体的两种DNA对照样品。从原始数据文件分析质量控制指标和关于常规程序的调查。结果表明覆盖范围的差异很大,但是原始数据文件中的变异等位基因频率符合预定义的变体等位基因频率。由于低质量的地区,发现了许多假阴性结果,这是没有报道的。建议披露可报告范围,可以产生可接受质量呼叫的靶向基因组区域的分数,以避免治疗决策中的任何误差。只有在应用和报告的基本质量控制,才能是一种可靠的技术。

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