Original article
T-cell clonality assessment by next-generation sequencing improves detection sensitivity in mycosis fungoides

Presented in poster format at the United States and Canadian Academy of Pathology Annual Meeting held in San Diego, CA on March 3, 2014.
https://doi.org/10.1016/j.jaad.2015.04.030Get rights and content
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Background

T-cell receptor (TCR) clonality assessment is a principal diagnostic test in the management of mycosis fungoides (MF). However, current polymerase chain reaction–based methods may produce ambiguous results, often because of low abundance of clonal T lymphocytes, resulting in weak clonal peaks that cannot be size-resolved by contemporary capillary electrophoresis (CE).

Objective

We sought to determine if next-generation sequencing (NGS)-based detection has increased sensitivity for T-cell clonality over CE-based detection in MF.

Methods

Clonality was determined by an NGS-based method in which the TCR-γ variable region was polymerase chain reaction amplified and the products sequenced to establish the identity of rearranged variable and joining regions.

Results

Of the 35 MF cases tested, 29 (85%) showed a clonal T-cell rearrangement by NGS, compared with 15 (44%) by standard CE detection. Three patients with MF had follow-up testing that showed identical, clonal TCR sequences in subsequent skin biopsy specimens.

Limitations

Clonal T-cell populations have been described in benign conditions; evidence of clonality alone, by any method, is not sufficient for diagnosis.

Conclusion

TCR clonality assessment by NGS has superior sensitivity compared with CE-based detection. Further, NGS enables tracking of specific clones across multiple time points for more accurate identification of recurrent MF.

Key words

cutaneous T-cell lymphoma
molecular diagnostics
mycosis fungoides
next-generation sequencing
T-cell clonality
T-cell receptor rearrangement

Abbreviations used

CE
capillary electrophoresis
CTCL
cutaneous T-cell lymphoma
MF
mycosis fungoides
NGS
next-generation sequencing
PCR
polymerase chain reaction
TCR
T-cell receptor

Cited by (0)

This project was funded by the Washington University Department of Pathology and Immunology.

Conflicts of interest: None declared.

Reprints not available from the authors.