| Literature DB >> 30566947 |
Pasquale Pisapia1, Umberto Malapelle1, Giancarlo Troncone2.
Abstract
The identification of non-small cell lung cancer (NSCLC) patients potentially responsive to targeted therapies relies on a number of relevant biomarkers, including EGFR, ALK, ROS-1, and PD-L1. Biomarker identification is most commonly based on surgical sample collection. However, when tissues are difficult to reach or when multiple analyses are necessary to monitor tumor progression and treatment response, liquid biopsy is a valid noninvasive alternative. This analysis, which is preferentially performed on circulating tumor DNA (ctDNA) extracted from plasma samples, has the major advantage of reducing the inherent risks and discomfort of tissue biopsy. However, a major disadvantage is that it yields only a low number of ctDNA targets. Thus, to avoid false-positive and false-negative results, it is important to adopt and validate technologies with high sensitivity and specificity in the pre-analytical phase of sampling. This review succinctly addresses the principal methodologies for analyzing plasma-derived ctDNA in NSCLC patients.Entities:
Keywords: Circulating tumor DNA; Digital polymerase chain reaction; EGFR; Liquid biopsy; Lung cancer; Next generation sequencing; Non-small cell lung cancer; Personalized medicine; Quantitative polymerase chain reaction
Mesh:
Substances:
Year: 2018 PMID: 30566947 DOI: 10.1159/000492710
Source DB: PubMed Journal: Acta Cytol ISSN: 0001-5547 Impact factor: 2.319