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将循环肿瘤 DNA 分析扩展到超低丰度突变:技术和挑战。

Extending Circulating Tumor DNA Analysis to Ultralow Abundance Mutations: Techniques and Challenges.

机构信息

Myeloma Research Group, Australian Center for Blood Diseases , Monash University , Melbourne , Victoria 3004 , Australia.

Malignant Haematology & Stem Cell Transplantation Service , Alfred Hospital , Melbourne , Victoria 3004 , Australia.

出版信息

ACS Sens. 2018 Mar 23;3(3):540-560. doi: 10.1021/acssensors.7b00953. Epub 2018 Feb 23.

DOI:10.1021/acssensors.7b00953
PMID:29441780
Abstract

Liquid biopsies that analyze circulating tumor DNA (ctDNA) hold great promise in the guidance of clinical treatment for various cancers. However, the innate characteristics of ctDNA make it a difficult target: ctDNA is highly fragmented, and found at very low concentrations, both in absolute terms and relative to wildtype species. Clinically relevant target sequences often differ from the wildtype species by a single DNA base pair. These characteristics make analyzing mutant ctDNA a uniquely difficult process. Despite this, techniques have recently emerged for analyzing ctDNA, and have been used in pilot studies that showed promising results. These techniques each have various drawbacks, either in their analytical capabilities or in practical considerations, which restrict their application to many clinical situations. Many of the most promising potential applications of ctDNA require assay characteristics that are not currently available, and new techniques with these properties could have benefits in companion diagnostics, monitoring response to treatment and early detection. Here we review the current state of the art in ctDNA detection, with critical comparison of the analytical techniques themselves. We also examine the improvements required to expand ctDNA diagnostics to more advanced applications and discuss the most likely pathways for these improvements.

摘要

液体活检分析循环肿瘤 DNA(ctDNA)在指导各种癌症的临床治疗方面具有巨大的潜力。然而,ctDNA 的固有特性使其成为一个难以攻克的目标:ctDNA 高度碎片化,并且无论在绝对值还是与野生型相比,其浓度都非常低。临床上相关的靶序列通常与野生型仅相差一个 DNA 碱基对。这些特性使得分析突变 ctDNA 成为一个非常困难的过程。尽管如此,最近还是出现了用于分析 ctDNA 的技术,并在显示出有前景的结果的初步研究中得到了应用。这些技术各自在分析能力或实际考虑方面都存在各种缺点,限制了它们在许多临床情况下的应用。ctDNA 的许多最有前途的潜在应用都需要目前尚未具备的检测特性,而具有这些特性的新技术在伴随诊断、监测治疗反应和早期检测方面可能具有优势。在这里,我们回顾了 ctDNA 检测的最新技术,对分析技术本身进行了批判性比较。我们还研究了将 ctDNA 诊断扩展到更先进的应用所需的改进,并讨论了这些改进最有可能的途径。

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