Optimizing Mutation and Fusion Detection in NSCLC by Sequential DNA and RNA Sequencing

Danielle Cohen; Liesbeth M Hondelink; Nienke Solleveld-Westerink; Sandra M Uljee; Dina Ruano; Anne-Marie Cleton-Jansen; Jan H von der Thüsen; S Rajen S Ramai; Pieter E Postmus; Jacob F Graadt van Roggen; Bart P C Hoppe; Pieter C Clahsen; Klaartje W Maas; Els J M Ahsmann; Alexandra Ten Heuvel; Frank Smedts; Ronald N van Rossem; Tom van Wezel

doi:10.1016/j.jtho.2020.01.019

Optimizing Mutation and Fusion Detection in NSCLC by Sequential DNA and RNA Sequencing

J Thorac Oncol. 2020 Jun;15(6):1000-1014. doi: 10.1016/j.jtho.2020.01.019. Epub 2020 Jan 31.

Authors

Danielle Cohen¹, Liesbeth M Hondelink², Nienke Solleveld-Westerink², Sandra M Uljee², Dina Ruano², Anne-Marie Cleton-Jansen², Jan H von der Thüsen², S Rajen S Ramai³, Pieter E Postmus³, Jacob F Graadt van Roggen⁴, Bart P C Hoppe⁵, Pieter C Clahsen⁶, Klaartje W Maas⁷, Els J M Ahsmann⁸, Alexandra Ten Heuvel⁹, Frank Smedts¹⁰, Ronald N van Rossem¹¹, Tom van Wezel²

Affiliations

¹ Department of Pathology, Leiden University Medical Centre (LUMC), Leiden, The Netherlands. Electronic address: d.cohen@lumc.nl.
² Department of Pathology, Leiden University Medical Centre (LUMC), Leiden, The Netherlands.
³ Department of Pulmonology, Leiden University Medical Centre (LUMC), Leiden, The Netherlands.
⁴ Department of Pathology, Alrijne Hospital, Leiderdorp, The Netherlands.
⁵ Department of Pulmonology, Alrijne Hospital, Leiderdorp, The Netherlands.
⁶ Department of Pathology, Haaglanden Medical Centre (HMC), Den Haag, The Netherlands.
⁷ Department of Pulmonology, Haaglanden Medical Centre (HMC), Den Haag, The Netherlands.
⁸ Department of Pathology, Groene Hart Hospital (GHZ), Gouda, The Netherlands.
⁹ Department of Pulmonology, Groene Hart Hospital (GHZ), Gouda, The Netherlands.
¹⁰ Department of Pathology, Reinier de Graaf gasthuis (RdGG), Delft, The Netherlands.
¹¹ Department of Pulmonology, Reinier de Graaf gasthuis (RdGG), Delft, The Netherlands.

PMID: 32014610
DOI: 10.1016/j.jtho.2020.01.019

Abstract

Introduction: Frequently, patients with locally advanced or metastatic NSCLC are screened for mutations and fusions. In most laboratories, molecular workup includes a multitude of tests: immunohistochemistry (ALK, ROS1, and programmed death-ligand 1 testing), DNA sequencing, in situ hybridization for fusion, and amplification detection. With the fast-emerging new drugs targeting specific fusions and exon-skipping events, this procedure harbors a growing risk of tissue exhaustion.

Methods: In this study, we evaluated the benefit of anchored, multiplexed, polymerase chain reaction-based targeted RNA sequencing (RNA next-generation sequencing [NGS]) in the identification of gene fusions and exon-skipping events in patients, in which no pathogenic driver mutation was found by DNA-based targeted cancer hotspot NGS (DNA NGS). We analyzed a cohort of stage IV NSCLC cases from both in-house and referral hospitals, consisting 38.5% cytology samples and 61.5% microdissected histology samples, mostly core needle biopsies. We compared molecular findings in a parallel workup (DNA NGS and RNA NGS, cohort 1, n = 198) with a sequential workup (DNA NGS followed by RNA NGS in selected cases, cohort 2, n = 192). We hypothesized the sequential workup to be the more efficient procedure.

Results: In both cohorts, a maximum of one oncogenic driver mutation was found per case. This is in concordance with large, whole-genome databases and suggests that it is safe to omit RNA NGS when a clear oncogenic driver is identified in DNA NGS. In addition, this reduced the number of necessary RNA NGS to only 53% of all cases. The tumors of never smokers, however, were enriched for fusions and exon-skipping events (32% versus 4% in former and current smokers, p = 0.00), and therefore benefited more often from the shorter median turnaround time of the parallel approach (15 d versus only 9 d in the parallel workup).

Conclusions: We conclude that sequentially combining DNA NGS and RNA NGS is the most efficient strategy for mutation and fusion detection in smoking-associated NSCLC, whereas for never smokers we recommend a parallel approach. This approach was shown to be feasible on small tissue samples including for cytology tests, can drastically reduce the complexity and cost of molecular workup, and also provides flexibility in the constantly evolving landscape of actionable targets in NSCLC.

Keywords: DNA sequencing; Molecular diagnostics; NSCLC; Next-generation sequencing; RNA sequencing.

MeSH terms

DNA
High-Throughput Nucleotide Sequencing
Humans
Lung Neoplasms* / genetics
Mutation
Protein-Tyrosine Kinases* / genetics
Proto-Oncogene Proteins / genetics
Sequence Analysis, RNA

Substances

Proto-Oncogene Proteins
DNA
Protein-Tyrosine Kinases