Whole-genome informed circulating tumor DNA analysis by multiplex digital PCR for disease monitoring in B-cell lymphomas: a proof-of-concept study

Zahra Haider; Tove Wästerlid; Linn Deleskog Spångberg; Leily Rabbani; Cecilia Jylhä; Birna Thorvaldsdottir; Aron Skaftason; Hero Nikdin Awier; Aleksandra Krstic; Anna Gellerbring; Anna Lyander; Moa Hägglund; Ashwini Jeggari; Georgios Rassidakis; Kristina Sonnevi; Birgitta Sander; Richard Rosenquist; Emma Tham; Karin E Smedby

doi:10.3389/fonc.2023.1176698

Whole-genome informed circulating tumor DNA analysis by multiplex digital PCR for disease monitoring in B-cell lymphomas: a proof-of-concept study

Front Oncol. 2023 Jun 2:13:1176698. doi: 10.3389/fonc.2023.1176698. eCollection 2023.

Authors

Zahra Haider¹, Tove Wästerlid^{2

3}, Linn Deleskog Spångberg², Leily Rabbani¹, Cecilia Jylhä^{1

4}, Birna Thorvaldsdottir¹, Aron Skaftason¹, Hero Nikdin Awier⁴, Aleksandra Krstic^{1

4}, Anna Gellerbring⁵, Anna Lyander⁵, Moa Hägglund⁵, Ashwini Jeggari⁵, Georgios Rassidakis^{6

7}, Kristina Sonnevi^{2

3}, Birgitta Sander⁸, Richard Rosenquist^{1

4

9}, Emma Tham^{1

4}, Karin E Smedby^{2

3}

Affiliations

¹ Department of Molecular Medicine and Surgery, Karolinska Institutet, Stockholm, Sweden.
² Department of Medicine, Division of Clinical Epidemiology, Karolinska Institutet and Karolinska University Hospital, Stockholm, Sweden.
³ Department of Hematology, Karolinska University Hospital, Stockholm, Sweden.
⁴ Department of Clinical Genetics, Karolinska University Hospital, Stockholm, Sweden.
⁵ Clinical Genomics Stockholm, Science for Life Laboratory, School of Engineering Sciences in Chemistry, Biotechnology and Health, Royal Institute of Technology, Stockholm, Sweden.
⁶ Department of Oncology-Pathology, Karolinska Institutet, Stockholm, Sweden.
⁷ Department of Clinical Pathology and Cancer Diagnostics, Karolinska University Laboratory, Stockholm, Sweden.
⁸ Department of Laboratory Medicine, Division of Pathology and Cancer Diagnostics, Karolinska Institutet and Karolinska University Hospital, Stockholm, Sweden.
⁹ Genomic Medicine Center Karolinska, Karolinska University Hospital, Stockholm, Sweden.

Abstract

Introduction: Analyzing liquid biopsies for tumor-specific aberrations can facilitate detection of measurable residual disease (MRD) during treatment and at follow-up. In this study, we assessed the clinical potential of using whole-genome sequencing (WGS) of lymphomas at diagnosis to identify patient-specific structural (SVs) and single nucleotide variants (SNVs) to enable longitudinal, multi-targeted droplet digital PCR analysis (ddPCR) of cell-free DNA (cfDNA).

Methods: In 9 patients with B-cell lymphoma (diffuse large B-cell lymphoma and follicular lymphoma), comprehensive genomic profiling at diagnosis was performed by 30X WGS of paired tumor and normal specimens. Patient-specific multiplex ddPCR (m-ddPCR) assays were designed for simultaneous detection of multiple SNVs, indels and/or SVs, with a detection sensitivity of 0.0025% for SV assays and 0.02% for SNVs/indel assays. M-ddPCR was applied to analyze cfDNA isolated from serially collected plasma at clinically critical timepoints during primary and/or relapse treatment and at follow-up.

Results: A total of 164 SNVs/indels were identified by WGS including 30 variants known to be functionally relevant in lymphoma pathogenesis. The most frequently mutated genes included KMT2D, PIM1, SOCS1 and BCL2. WGS analysis further identified recurrent SVs including t(14;18)(q32;q21) (IGH::BCL2), and t(6;14)(p25;q32) (IGH::IRF4). Plasma analysis at diagnosis showed positive circulating tumor DNA (ctDNA) levels in 88% of patients and the ctDNA burden correlated with baseline clinical parameters (LDH and sedimentation rate, p-value <0.01). While clearance of ctDNA levels after primary treatment cycle 1 was observed in 3/6 patients, all patients analyzed at final evaluation of primary treatment showed negative ctDNA, hence correlating with PET-CT imaging. One patient with positive ctDNA at interim also displayed detectable ctDNA (average variant allele frequency (VAF) 6.9%) in the follow-up plasma sample collected 2 years after final evaluation of primary treatment and 25 weeks before clinical manifestation of relapse.

Conclusion: In summary, we demonstrate that multi-targeted cfDNA analysis, using a combination of SNVs/indels and SVs candidates identified by WGS analysis, provides a sensitive tool for MRD monitoring and can detect lymphoma relapse earlier than clinical manifestation.

Keywords: CtDNA; IGH-BCL2 translocation; cell-free DNA (cfDNA); droplet digital (ddPCR); liquid biopsy; lymphoma; measurable (minimal) residual disease (MRD); whole genome sequence (WGS).

Copyright © 2023 Haider, Wästerlid, Spångberg, Rabbani, Jylhä, Thorvaldsdottir, Skaftason, Awier, Krstic, Gellerbring, Lyander, Hägglund, Jeggari, Rassidakis, Sonnevi, Sander, Rosenquist, Tham and Smedby.

Grants and funding

The present study was partly funded by Region Stockholm (FoUI-973659, ET; FoUI-962423, RR), the Swedish Cancer Society (22 2451, ET; 19 0425, RR), the Swedish Childhood Cancer Fund (KP2021-0017 and TJ2021-0125, ET), Stockholm County Council (KES), Radiumhemmet Research Fund (KES; 194133, RR), the Swedish Research Council (2020-01750, RR) and the Knut and Alice Wallenberg Foundation (2016.0373, RR). Clinical postdoctoral appointment of TW was supported by Region Stockholm.