Next-Generation Sequencing Workflow for NSCLC Critical Samples Using a Targeted Sequencing Approach by Ion Torrent PGM™ Platform

被引:32
|
作者
Vanni, Irene [1 ]
Coco, Simona [1 ]
Truini, Anna [1 ,2 ]
Rusmini, Marta [3 ]
Dal Bello, Maria Giovanna [1 ]
Alama, Angela [1 ]
Banelli, Barbara [4 ]
Mora, Marco [5 ]
Rijavec, Erika [1 ]
Barletta, Giulia [1 ]
Genova, Carlo [1 ]
Biello, Federica [1 ]
Maggioni, Claudia [1 ]
Grossi, Francesco [1 ]
机构
[1] IRCCS AOU San Martino IST, Natl Inst Canc Res, Lung Canc Unit, I-16132 Genoa, Italy
[2] Univ Genoa, IRCCS AOU San Martino IST, Natl Inst Canc Res, Dept Internal Med & Med Specialties DIMI, I-16132 Genoa, Italy
[3] Giannina Gaslini Inst, IRCCS, Mol Genet Lab, I-16148 Genoa, Italy
[4] IRCCS AOU San Martino IST, Natl Inst Canc Res, Lab Tumor Epigenet, I-16132 Genoa, Italy
[5] IRCCS AOU San Martino IST, Natl Inst Canc Res, Dept Pathol, I-16132 Genoa, Italy
关键词
next-generation sequencing; NGS workflow; NSCLC; Ion Torrent PGM; FFPE; cfDNA; WHOLE-GENOME AMPLIFICATION; CELL LUNG-CANCER; INTRATUMOR HETEROGENEITY; DNA QUANTIFICATION; MUTATION DETECTION; GENE-MUTATIONS; POLYMORPHISMS; PCR; PERFORMANCE; STANDARDS;
D O I
10.3390/ijms161226129
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Next-generation sequencing (NGS) is a cost-effective technology capable of screening several genes simultaneously; however, its application in a clinical context requires an established workflow to acquire reliable sequencing results. Here, we report an optimized NGS workflow analyzing 22 lung cancer-related genes to sequence critical samples such as DNA from formalin-fixed paraffin-embedded (FFPE) blocks and circulating free DNA (cfDNA). Snap frozen and matched FFPE gDNA from 12 non-small cell lung cancer (NSCLC) patients, whose gDNA fragmentation status was previously evaluated using a multiplex PCR-based quality control, were successfully sequenced with Ion Torrent PGM (TM). The robust bioinformatic pipeline allowed us to correctly call both Single Nucleotide Variants (SNVs) and indels with a detection limit of 5%, achieving 100% specificity and 96% sensitivity. This workflow was also validated in 13 FFPE NSCLC biopsies. Furthermore, a specific protocol for low input gDNA capable of producing good sequencing data with high coverage, high uniformity, and a low error rate was also optimized. In conclusion, we demonstrate the feasibility of obtaining gDNA from FFPE samples suitable for NGS by performing appropriate quality controls. The optimized workflow, capable of screening low input gDNA, highlights NGS as a potential tool in the detection, disease monitoring, and treatment of NSCLC.
引用
收藏
页码:28765 / 28782
页数:18
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