Complex Karyotype Detection in Chronic Lymphocytic Leukemia: A Comparison of Parallel Cytogenetic Cultures Using TPA and IL2+DSP30 from a Single Center

Author:

Kamaso Joanna12,Puiggros Anna12ORCID,Salido Marta12,Melero Carme12,Rodríguez-Rivera María12,Gimeno Eva34,Martínez Laia5,Arenillas Leonor12ORCID,Calvo Xavier12ORCID,Román David12,Abella Eugènia3,Ramos-Campoy Silvia12,Lorenzo Marta12,Ferrer Ana12,Collado Rosa6ORCID,Moro-García Marco Antonio7ORCID,Espinet Blanca12ORCID

Affiliation:

1. Molecular Cytogenetics and Hematological Cytology Laboratories, Pathology Department, Hospital del Mar, 08003 Barcelona, Spain

2. Translational Research on Hematological Neoplasms Group, Cancer Research Program, Hospital del Mar Research Institute (HMRI), 08003 Barcelona, Spain

3. Department of Hematology, Hospital del Mar, 08003 Barcelona, Spain

4. Applied Clinical Research in Hematological Malignances Group, Cancer Research Program, Hospital del Mar Research Institute (HMRI), 08003 Barcelona, Spain

5. Hematology Service, Hospital Universitari Sant Joan de Reus, 43204 Reus, Spain

6. Department of Hematology, Consorcio Hospital General Universitario Valencia, 46014 Valencia, Spain

7. Laboratory Medicine Department, Hospital Universitario Central de Asturias, 33011 Oviedo, Spain

Abstract

Current CLL guidelines recommend a two parallel cultures assessment using TPA and IL2+DSP30 mitogens for complex karyotype (CK) detection. Studies comparing both mitogens for CK identification in the same cohort are lacking. We analyzed the global performance, CK detection, and concordance in the complexity assessment of two cytogenetic cultures from 255 CLL patients. IL2+DSP30 identified more altered karyotypes than TPA (50 vs. 39%, p = 0.031). Moreover, in 71% of those abnormal by both, IL2+DSP30 identified more abnormalities and/or abnormal metaphases. CK detection was similar for TPA and IL2+DSP30 (10% vs. 11%). However, 11/33 CKs (33%) were discordant, mainly due to the detection of a normal karyotype or no metaphases in the other culture. Patients requiring treatment within 12 months after sampling (active CLL) displayed significantly more CKs than those showing a stable disease (55% vs. 12%, p < 0.001). Disease status did not impact cultures’ concordance (κ index: 0.735 and 0.754 for stable and active). Although CK was associated with shorter time to first treatment (TTFT) using both methods, IL2+DSP30 displayed better accuracy than TPA for predicting TTFT (C-index: 0.605 vs. 0.580, respectively). In summary, the analysis of two parallel cultures is the best option to detect CKs in CLL. Nonetheless, IL2+DSP30 could be prioritized above TPA to optimize cytogenetic assessment in clinical practice.

Funder

Generalitat de Catalunya

Gilead Sciences Fellowship

Fundación Española de Hematología y Hemoterapia (FEHH)-AstraZeneca

Publisher

MDPI AG

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4. (2024, April 29). Chronische Lymphatische Leukämie (CLL) Onkopedia. Available online: https://www.onkopedia.com/de/onkopedia/guidelines/chronische-lymphatische-leukaemie-cll/@@guideline/html/index.html.

5. Patients with chronic lymphocytic leukemia and complex karyotype show an adverse outcome even in absence of TP53/ATM FISH deletions;Puiggros;Oncotarget,2017

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