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循环肿瘤DNA:诊断实验室中的分析前验证与质量控制

Circulating tumoral DNA: Preanalytical validation and quality control in a diagnostic laboratory.

作者信息

Nikolaev Sergey, Lemmens Laure, Koessler Thibaud, Blouin Jean-Louis, Nouspikel Thierry

机构信息

Molecular and Genomic Diagnostic Laboratory, Service of Medical Genetics, Department of Genetic Medicine, Laboratory Medicine and Pathology, University Hospitals of Geneva, CH-1211 Geneva, Switzerland.

Department of Oncology, University Hospitals of Geneva, Geneva, Switzerland.

出版信息

Anal Biochem. 2018 Feb 1;542:34-39. doi: 10.1016/j.ab.2017.11.004. Epub 2017 Nov 11.

Abstract

We present the results of our technical validation process in establishing the analysis of circulating tumor DNA (ctDNA) as a diagnostic tool. Like most cells in our body, tumor cells shed DNA in the blood flow. Analysis of ctDNA mutational content can provide invaluable information on the genetic makeup of a tumor, and assist oncologists in deciding on therapy, or in following residual disease. However, low absolute amounts of circulating DNA and low tumor fraction constitute formidable analytical challenges. A key step is to avoid contamination with genomic DNA from cell lysis. Several brands of specialized blood collection tubes are available to prevent leukocyte lysis. We show that they are not equally efficient, depending on storage temperature and time before plasma preparation. We report our analysis of preanalytical factors pertaining to ctDNA analysis (tubes, transportation time, temperature) and our conclusions in terms of instructions to prescribing physicians. We also stress the importance of proper DNA quality control and compare several methods, including a differential amplicon length PCR technique which allows determination of multiple QC parameters from minimal amounts of DNA. Altogether, these data provide useful practical information to diagnostic laboratories wishing to implement the assay of ctDNA in clinical practice.

摘要

我们展示了将循环肿瘤DNA(ctDNA)分析确立为一种诊断工具的技术验证过程的结果。与我们体内的大多数细胞一样,肿瘤细胞会在血流中释放DNA。对ctDNA突变含量的分析可以提供有关肿瘤基因组成的宝贵信息,并帮助肿瘤学家确定治疗方案或追踪残留疾病。然而,循环DNA的绝对量低和肿瘤比例低构成了巨大的分析挑战。关键步骤是避免细胞裂解产生的基因组DNA污染。有几种专门的采血管品牌可用于防止白细胞裂解。我们表明,根据储存温度和制备血浆前的时间不同,它们的效率并不相同。我们报告了我们对与ctDNA分析相关的分析前因素(采血管、运输时间、温度)的分析以及我们对给开处方医生的建议的结论。我们还强调了适当的DNA质量控制的重要性,并比较了几种方法,包括一种差异扩增子长度PCR技术,该技术可以从极少量的DNA中确定多个质量控制参数。总之,这些数据为希望在临床实践中实施ctDNA检测的诊断实验室提供了有用的实用信息。

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