Dear Editor,
Fluorescent in situ hybridization (FISH), metaphase cytogenetics, and single nucleotide polymorphism (SNP) microarray have long been the standard assays for disease diagnostics and subtyping of multiple myeloma. With the advent of next generation sequencing (NGS), our understanding of the genomic landscape in multiple myeloma has been expanded. Recent data show that NGS-based myeloma-targeted assays can identify immunoglobulin heavy chain (IGH) translocations, copy number alterations, as well as somatic mutations1. Comprehensive genomic profiling of multiple myeloma is becoming increasingly important for individual risk stratification and therapeutic guidance2. Therefore, NGS-based myeloma-targeted assays will gradually replace current standard methods in clinical practice.
In addition to initial genomic profiling of multiple myeloma, the depth of treatment response—measured as minimal residual disease (MRD)—is an important prognostic factor. MRD evaluation with multicolor flow cytometry or immunoglobulin V(D)J sequencing to assess depth of treatment response and to inform clinical decisions is becoming standard in many centers across the USA3,4.
Recently, we conducted a head-to-head comparison of an NGS-based multiple myeloma-targeted assay (named “myTYPE”) and found that the targeted assay had a high concordance, >99% sensitivity and specificity, for detection IGH translocations and copy number alterations compared to FISH and SNP microarray1. In addition, the NGS assay captures somatic mutations in 120 genes that are recurrent and relevant in multiple myeloma1,5,6,7,8. Here, as a follow-up, we assessed whether the targeted NGS assay can detect patient-specific V(D)J clonotypes at diagnosis, something that is required for subsequent longitudinal MRD tracking.
The commercially available LymphoTrack assays (i.e. IGH Leader, FR1, FR2 and FR3; Invivoscribe Inc, San Diego, CA) and our custom capture next NGS-based panel were used to sequence 74 multiple myeloma samples1,9,10. Polymerase chain reaction amplification of the IGH variable region followed by NGS to a target read depth of >20,000 and clonality calling was performed using LymphoTrack as previously described10. The myTYPE assay includes canonical IGH locus was included to capture IGH (14q32) rearrangements11. This locus also includes the V(D)J regions of the IGH gene. The MiXCR algorithm was used to reconstruct the V(D)J region from short-read data (Fig. 1)9,12,13. The V(D)J clonotypes detected through the targeted NGS panel were then compared to the clonotypes detected in the same samples using the LymphoTrack assay10. The study was approved by the Institutional Review Board and all patients were seen at Memorial Sloan Kettering Cancer Center and had consented to the tissue acquisition protocol.
In 74 samples with a clonal V(D)J sequence detected by Lymphotrack; using myTYPE, the same clonal V(D)J sequence was found in 70 samples (95%). In all 70 samples, the CDR3 sequence detected with myTYPE was identical to the CDR3 sequence reported by LymphoTrack. We went on to examine in detail the four patients where no clonal sequence was detected with myTYPE. There was an adequate sequencing coverage of the IGH region in these patients, the median IGH coverage ranged between 671 and 1043× in the four samples compared to 842× in the whole cohort. The four samples had bone marrow plasma cell infiltration of 20% or higher and the sample purity ranged between 64 and 84%, estimated through the ASCAT algorithm on the SNP array samples and an in-house algorithm based on the NGS results14. One patient had an incomplete V(D)J rearrangement identified by LymphoTrack, without a CDR3 sequence that could be identified by MiXCR. This patient had a hyperdiploid karyotype and a detectable IgG lambda monoclonal protein in serum and no IGH translocation detected through FISH or NGS. In the remaining three patients, LymphoTrack identified a productive V(D)J CDR3 sequence as the dominant clonotype. In two of these patients, we could identify the dominant CDR3 sequence in raw sequence data (i.e. FASTQ files) from myTYPE, although it was not called by MiXCR. In the fourth case, the NGS output was successful and the V(D)J clonotype was detected with LymphoTrack but not by with MiXCR or in raw sequence data. Further improvements in algorithm design are expected to increase capture rates close to the current standard of amplifying the entire V(D)J region on a single sequencing read (e.g., LymphoTrack).
In the process of B-cell development, the V(D)J region of the IGH is rearranged to create different combinations of the segments in the variable region of the gene resulting in immunoglobulin with different targets. The large number of variations of the V(D)J sequence and the subsequent somatic hypermutation can however negatively affect the annealing of primers and thus decrease the capture rate. The two available commercial assays have overcome this by including multiple probes primers at various distances from the immunoglobulin variable regions (LymphoTrack) or including probes that cover a wide variety of V(D)J combinations including incomplete rearrangements (ClonoSEQ)9,15. Using standard short-read sequencing data, the algorithm MiXCR aligns reads mapping to a library of reference germline V, D, J, and C gene sequences to assemble full-length clonotypes. The algorithm can correct for mismatches and indels that occur during hypermutation12. All of the assays routinely used for V(D)J sequencing in the MRD setting require baseline characterization to identify a clonotype for tracking. V(D)J sequencing has an advantage in that the V(D)J clonotypes are stable over time and do not seem to undergo further somatic hypermutation after the diagnosis of multiple myeloma13. Thus, DNA sequencing of the V(D)J region is optimal for disease tracking provided that the baseline V(D)J clonotypes are known.
In summary, NGS profiling of multiple myeloma using a myeloma-targeted assay is comparable or better than standard methods, e.g., FISH and SNP microarray, for detecting IGH translocations and copy number alterations1. Here, we additionally show that by including the IGH locus, V(D)J clonotypes can be detected using targeted sequencing. Overall, our findings suggest that baseline genomic profiling–including IGH translocations, copy number alterations, recurrent somatic mutations, as well as patient-specific V(D)J clonotypes relevant for longitudinal MRD tracking—can all be captured using a single myeloma-targeted NGS assay.
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Acknowledgements
Funding support for this publication was provided by the Multiple Myeloma Research Foundation (MMRF); The Perelman Family Foundation: the Swedish Research Council (2015-00564); and the Memorial Sloan Kettering Core Grant (P30 CA008748).
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M.H., E.H.R., and O.L. designed the study, M.H., E.H.R., V.Y., M.A., C.H., M.H.S., F.M., and O.L. collected, analyzed, and interpreted the data, M.H., E.H.R., and O.L. wrote the paper. All authors provided critical input on the results and gave final approval of the manuscript.
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M.H. has received funding from the Multiple Myeloma Research Foundation and the Swedish Research Council and honoraria from Intellisphere, LLC. E.P. is a Josie Robertson Investigator, an EHA Fellow, and an ASH Scholar. O.L. has received research funding from: National Institutes of Health (NIH), U.S. Food and Drug Administration (FDA), Multiple Myeloma Research Foundation (MMRF), International Myeloma Foundation (IMF), Leukemia and Lymphoma Society (LLS), The Perelman Family Foundation, Rising Tides Foundation, Amgen, Celgene, Janssen, Takeda, Glenmark, Seattle Genetics, Karyopharm; Honoraria/ad boards: Adaptive, Amgen, Binding Site, BMS, Celgene, Cellectis, Glenmark, Janssen, Juno, Pfizer; and serves on Independent Data Monitoring Committees (IDMCs) for clinical trials lead by Takeda, Merck, Janssen, and Theradex. There is a pending patent application regarding the myTYPE assay (authors M.H., E.P. and O.L.). The remaining authors declare no relevant conflicts of interest.
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Hultcrantz, M., Rustad, E.H., Yellapantula, V. et al. Baseline VDJ clonotype detection using a targeted sequencing NGS assay: allowing for subsequent MRD assessment. Blood Cancer J. 10, 76 (2020). https://doi.org/10.1038/s41408-020-00343-w
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DOI: https://doi.org/10.1038/s41408-020-00343-w
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