| Literature DB >> 33811533 |
Ivonne Vazquez1,2, Natalia Papaleo1,3,4, Joan Lop1, Anna Puiggros1, Blanca Sanchez-Gonzalez5, Ramon Diez-Feijoo5, Eva Gimeno5, Marcio Andrade-Campos5, Antonio Salar5, Blanca Espinet1, Marta Salido1, Gustavo Tapia6, Joaquim Carreras7, Ana Ferrer1,4, Leonor Arenillas1, Xavier Calvo1, Luis Colomo8,9.
Abstract
MYC rearrangements (MYC-R) confer unfavorable prognosis to large B-cell lymphomas (LBCL). Because of the low incidence of such genetic alteration, surrogates to screen MYC-R may be useful in daily practice. Previous studies suggested that clone 1A9-1 of LMO2 loss may be a good predictor for the presence of MYC-R in LBCL. The present study examines the utility of LMO2 clone SP51. For this purpose, we have analyzed 20 Burkitt lymphomas and 325 LBCL. Among them, 245 cases were studied prospectively using whole tissue sections, and 100 retrospectively by tissue microarrays. The cohort of CD10-positive prospective cases achieved the best results. Lack of LMO2 SP51 expression predicted the presence of MYC-R with high specificity, accuracy, positive and negative predictive value (PPV/NPV), and positive and negative likelihood ratios (PLR/NLR). Compared with MYC protein expression, LMO2 SP51 obtained significantly higher specificity, accuracy, PPV, and PLR (94%, 91%, 85%, and 14.33 vs 73%, 77%, 56%, and 3.26, respectively), and similar NPV and NLR (92% and 0.22 vs 95% and 0.12). Compared with LMO2 clone 1A9-1, the sensitivity of LMO2 SP51 was lower (79% vs 89%). We conclude that LMO2 SP51 may be a useful marker to screen MYC-R in CD10-positive LBCL.Entities:
Keywords: Immunohistochemistry; LMO2; Large B-cell lymphoma; MYC
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Year: 2021 PMID: 33811533 DOI: 10.1007/s00428-021-03091-9
Source DB: PubMed Journal: Virchows Arch ISSN: 0945-6317 Impact factor: 4.064