Molecular diagnosis of T-cell lymphoma: a correlative study of PCR-based T-cell clonality assessment and targeted NGS

Author:

Syrykh Charlotte1ORCID,Gorez Pauline1,Péricart Sarah1,Grand David1,Escudié Frédéric1,Cabarrou Bastien2,Obéric Lucie3ORCID,Ysebaert Loïc34,Lamant Laurence1,Laurent Camille14,Evrard Solène M.14ORCID,Brousset Pierre14ORCID

Affiliation:

1. Pathology Department, Institut Universitaire du Cancer-Oncopole, CHU Toulouse, Labex TOUCAN, Toulouse, France;

2. Biostatistics Department, Institut Claudius Regaud, Institut Universitaire du Cancer-Oncopole, Toulouse, France;

3. Hematology Department, Institut Universitaire du Cancer-Oncopole, Toulouse, France; and

4. Institut National de la Santé et de la Recherche Médicale UMR1037, Centre de Recherches en Cancérologie de Toulouse, Université de Toulouse III Paul-Sabatier, Toulouse, France

Abstract

Abstract Immunomorphological diagnosis of T-cell lymphoma (TCL) may be challenging, especially on needle biopsies. Multiplex polymerase chain reaction (PCR) assays to assess T-cell receptor (TCR) gene rearrangements are now widely used to detect T-cell clones and provide diagnostic support. However, PCR assays detect only 80% of TCL, and clonal lymphocyte populations may also appear in nonneoplastic conditions. More recently, targeted next-generation sequencing (t-NGS) technologies have been deployed to improve lymphoma classification. To the best of our knowledge, the comparison of these techniques’ performance in TCL diagnosis has not been reported yet. In this study, 82 TCL samples and 25 nonneoplastic T-cell infiltrates were divided into 2 cohorts (test and validation) and analyzed with both multiplex PCR and t-NGS to investigate TCR gene rearrangements and somatic mutations, respectively. The detection of mutations appeared to be more specific (100.0%) than T-cell clonality assessment (41.7%-45.5%), whereas no differences were observed in terms of sensitivity (95.1%-97.4%). Furthermore, t-NGS provided a reliable basis for TCL diagnosis in samples with partially degraded DNA that was impossible to assess with PCR. Finally, although multiplex PCR assays appeared to be less specific than t-NGS, both techniques remain complementary, as PCR recovered some t-NGS negative cases.

Publisher

American Society of Hematology

Subject

Hematology

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